International Review of Cytology, A Survey of Cell Biology, Vol. 260

International Review of A Survey of Cytology Cell Biology VOLUME 260 SERIES EDITORS Geoffrey H. Bourne James F. Dan...

Author: Kwang W. Jeon

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International Review of

A Survey of

Cytology Cell Biology VOLUME 260

SERIES EDITORS Geoffrey H. Bourne James F. Danielli Kwang W. Jeon Martin Friedlander Jonathan Jarvik

1949–1988 1949–1984 1967– 1984–1992 1993–1995

EDITORIAL ADVISORY BOARD Isaiah Arkin Eve Ida Barak Peter L. Beech Howard A. Bern Robert A. Bloodgood Dean Bok Hiroo Fukuda Ray H. Gavin Siamon Gordon May Griffith William R. Jeffery

Keith Latham Wallace F. Marshall Bruce D. McKee Michael Melkonian Keith E. Mostov Andreas Oksche Thoru Pederson Manfred Schliwa Teruo Shimmen Robert A. Smith Wildred D. Stein Nikolai Tomilin

International Review of A Survey of

Cytology Cell Biology

Edited by

Kwang W. Jeon Department of Biochemistry University of Tennessee Knoxville, Tennessee

VOLUME 260

AMSTERDAM • BOSTON • HEIDELBERG • LONDON NEW YORK • OXFORD • PARIS • SAN DIEGO SAN FRANCISCO • SINGAPORE • SYDNEY • TOKYO Academic Press is an imprint of Elsevier

Front Cover Photograph: Courtesy of Dr. Sarah Mackay and Dr. Rob Smith, Faculty of Biomedical and Life Sciences, University of Glasgow, United Kingdom.

Academic Press is an imprint of Elsevier 525 B Street, Suite 1900, San Diego, California 92101-4495, USA 84 Theobald’s Road, London WC1X 8RR, UK

This book is printed on acid-free paper. Copyright ß 2007, Elsevier Inc. All Rights Reserved.

No part of this publication may be reproduced or transmitted in any form or by any means, electronic or mechanical, including photocopy, recording, or any information storage and retrieval system, without permission in writing from the Publisher. The appearance of the code at the bottom of the first page of a chapter in this book indicates the Publisher’s consent that copies of the chapter may be made for personal or internal use of specific clients. This consent is given on the condition, however, that the copier pay the stated per copy fee through the Copyright Clearance Center, Inc. (www.copyright.com), for copying beyond that permitted by Sections 107 or 108 of the U.S. Copyright Law. This consent does not extend to other kinds of copying, such as copying for general distribution, for advertising or promotional purposes, for creating new collective works, or for resale. Copy fees for pre-2007 chapters are as shown on the title pages. If no fee code appears on the title page, the copy fee is the same as for current chapters. 0074-7696/2007 $35.00 Permissions may be sought directly from Elsevier’s Science & Technology Rights Department in Oxford, UK: phone: (þ44) 1865 843830, fax: (þ44) 1865 853333, E-mail: [email protected]. You may also complete your request on-line via the Elsevier homepage (http://elsevier.com), by selecting ‘‘Support & Contact’’ then ‘‘Copyright and Permission’’ and then ‘‘Obtaining Permissions.’’ For information on all Elsevier Academic Press publications visit our Web site at www.books.elsevier.com ISBN-13: 978-0-12-374114-1 ISBN-10: 0-12-374114-9 PRINTED IN THE UNITED STATES OF AMERICA 07 08 09 10 9 8 7 6 5 4 3 2 1

CONTENTS

Contributors ......................................................................................

vii

Cell Proliferation in Pathogenesis of Esophagogastric Lesions in Pigs Milijana Knezˇevic´, Sanja Aleksic´-Kovacˇevic´, and Zoran Aleksic´ I. II. III. IV.

Introduction ............................................................................... Morphofunctional Features of Swine Stomach ..................................... Esophagogastric Ulcer in Swine....................................................... Concluding Remarks .................................................................... References ................................................................................

2 3 10 27 27

Molecular Mechanism of Phase I and Phase II Drug-Metabolizing Enzymes: Implications for Detoxification Takashi Iyanagi I. Introduction ............................................................................... II. Phase I: NADPH-Cytochrome P450 Reductase (P450R)/Cytochrome P450 (P450) System .................................................................... III. Phase II: UDP-Glucuronosyltransferase (UGT) ..................................... IV. Coordinated Biotransformation by P450 and UGT ................................. V. Concluding Remarks .................................................................... References ................................................................................ v

35 36 56 73 88 89

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CONTENTS

Effects of Growth Factors on Testicular Morphogenesis Sarah Mackay and Robert A. Smith I. II. III. IV. V. VI. VII. VIII.

Introduction............................................................................... Comparative Testicular Morphogenesis ............................................. Cell Migration............................................................................. Vascular Development .................................................................. Proliferation............................................................................... Control of Cell Phenotype/Differentiation............................................ Experimental Manipulations In Vitro ................................................. Concluding Remarks .................................................................... References ................................................................................

113 114 118 125 128 139 153 158 161

Flagellar Length Control in Chlamydomonas—A Paradigm for Organelle Size Regulation Kimberly A. Wemmer and Wallace F. Marshall I. II. III. IV.

Introduction............................................................................... Size of Organelles ....................................................................... Models for Flagellar Length Control System ....................................... Conclusion: What Have We Learned from Flagellar Length Control?.......... References ................................................................................

175 176 192 203 207

Molecular Mechanism and Evolutional Significance of Epithelial–Mesenchymal Interactions in the Body- and Tail-Dependent Metamorphic Transformation of Anuran Larval Skin Katsutoshi Yoshizato I. II. III. IV. V.

Introduction............................................................................... Anuran Skin Remodeling and Metamorphosis ..................................... Epithelial–Mesenchymal Interactions and Larval Skin Remodeling............. Genes Involved in Anuran Tissue Remodeling ..................................... Concluding Remarks .................................................................... References ................................................................................

214 217 234 243 252 253

Index ..............................................................................................

261

CONTRIBUTORS

Numbers in parentheses indicate the pages on which the authors’ contributions begin.

Zoran Aleksic´ (1), Department of Pathology, Faculty of Veterinary Medicine, University of Belgrade, 11000 Belgrade, Serbia Sanja Aleksic´-Kovacˇevic´ (1), Department of Pathology, Faculty of Veterinary Medicine, University of Belgrade, 11000 Belgrade, Serbia Takashi Iyanagi (35), Biometal Science Laboratory, RIKEN SPring-8 Center, Harima Institute, Hyogo 679-5148, Japan Milijana Knezˇevic´ (1), Department of Pathology, Faculty of Veterinary Medicine, University of Belgrade, 11000 Belgrade, Serbia Sarah Mackay (113), Division of Neuroscience and Biomedical Systems, Institute of Biomedical and Life Sciences, University of Glasgow, Glasgow, UK G12 8QQ Wallace F. Marshall (175), Department of Biochemistry, University of California, San Francisco, San Francisco, California 94158 Robert A. Smith (113), Division of Neuroscience and Biomedical Systems, Institute of Biomedical and Life Sciences, University of Glasgow, Glasgow, UK G12 8QQ Kimberly A. Wemmer (175), Department of Biochemistry, University of California, San Francisco, San Francisco, California 94158 Katsutoshi Yoshizato (213), Department of Biological Science, Graduate School of Science, Hiroshima University, Higashihiroshima, 7398526, Japan

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Cell Proliferation in Pathogenesis of Esophagogastric Lesions in Pigs Milijana Knezˇevic´, Sanja Aleksic´‐Kovacˇevic´, and Zoran Aleksic´ Department of Pathology, Faculty of Veterinary Medicine, University of Belgrade, 11000 Belgrade, Serbia

Esophagogastric ulcer is an independent disease in swine that is characterized by ulcerous autodigestion of the cutaneous mucosa, which does not exhibit a tendency to recover, but, on the contrary, a tendency toward severe hemorrhaging, with a predominantly lethal outcome. Since it develops in the part of the stomach that is morphologically and functionally different from other glandular mucosa, it was questioned earlier whether it could be a peptic ulcer based on its nature. Spontaneous ulcers, usually of the stomach, commonly occur in many domestic animals. Some of these lesions are chronic and they may occur in either the glandular or squamous‐lined regions of the stomach. As with the human disease, the pathogenesis in domestic animals is multifactorial, poorly understood, and variable between and within species. Environmental stress and dietary factors are very important in the ulcer disease in swine. It has been shown that the Helicobacter spp. is strongly associated with naturally occurring ulcer and preulcer lesions of the pars esophagea in swine, which raises the possibility that Helicobacter spp. is an important factor in the pathogenesis of these lesions. The dynamics of the development of esophagogastric ulcers imply hyperplastic lesions (parakeratosis and hyperkeratosis), keratolysis, erosions, peptic necrosis, and the development of ulcers with all the characteristics of peptic ulcerations in other localities. In addition, K6 is expressed in association with the mucosal changes. The pattern of the intermediate filaments of keratin suggests that epithelial proliferation, which leads to visible hyperkeratosis, constitutes the essence of gastric ulcers in swine. KEY WORDS: Swine, Esophagogastric ulcer, Parakeratosis, Hyperkeratosis, Keratin. ß 2007 Elsevier Inc.

International Review of Cytology, Vol. 260 Copyright 2007, Elsevier Inc. All rights reserved.

1

0074-7696/07 $35.00 DOI: 10.1016/S0074-7696(06)60001-6

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I. Introduction Esophagogastric ulcer is an independent disease in swine that is characterized by ulcerous autodigestion of the cutaneous mucosa, which does not exhibit a tendency to recover, but does exhibit a tendency toward severe hemorrhaging, with a predominantly lethal outcome. Since it develops in the part of the stomach that is morphologically and functionally diVerent from other glandular mucosa, it was questioned earlier whether it could be a peptic ulcer based on its nature. These dilemmas stemmed from the belief that peptic ulcerations can develop only in the duodenum and the glandular part of the stomach. However, peptic ulcerations today imply ‘‘holes in the mucosa’’ in any part of the gastrointestinal tract that is exposed to acidopeptic secretion. The morphological similarity between peptic ulcers in humans and in swine does not also imply an identical etiopathogenesis, although it can be assumed that there are certain common mechanisms of this multifactorial disease. With the exception of the epithelium, which has been aVected (squamous stratified glandless epithelium of the esophageal region), all morphological manifestations are identical to peptic ulcerations in other animal species and in humans. It is known that peptic ulcerations in humans and other animals are usually localized in the duodenum, the first portion of the stomach, usually the antrum, at the gastroesophageal junction, in the setting of the gastroesophageal reflux or Barrett’s esophagus, within the margins of a gastrojejunostomy, in the duodenum, stomach, and/or jejunum of patients with Zollinger–Ellison syndrome, and within or adjacent to an ileal Meckel diverticulum that contains ectopic gastric mucosa (Kumar et al., 2005), as opposed to swine, in which under natural and experimental conditions, ulcers predominantly develop in the pars esophagica. The most logical explanation for this localization is the fact that the squamous stratified epithelium of the esophageal part of the stomach of swine does not secrete mucoproteins, which weaken the natural mechanisms of defense from acidopeptic digestion. An ulcer of the esophageal part of the swine stomach was described for the first time in the United States in 1951, which was followed by more intensive investigations of its incidence in countries all over the world. Data during that period indicate that ulcers were present in Belgium in 4.7% of all examined swine, in Ireland in 53% (Muggenburg et al., 1964), and in the United States in 13.25–22% (GriYng, 1963). In Slovenia the incidence of this disease was followed in swine in intensive breeding conditions from 1963 until 1965, and a frequency of 0.9–12.68% was established (Sˇenk and Sˇabec, 1965). Numerous papers report that the incidence of this ulcer is most frequent in swine with a body mass of 40–90 kg (Bisson, 1967; Kowalczyk, 1970; Sˇenk, 1978). However, there are also data on frequent findings of esophagogastric

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ulcers in far younger swine, aged only 14 days (Curtin et al., 1963), or on the occurrence of ulcers on the pars pylorica of newborn piglets (Rothenbacher et al., 1963). According to certain references, ulcers are most frequent in swine with a body mass of up to 60 kg; this incidence declines in swine of 70–100 kg and again increases in swine with body mass over 100 kg. It has been observed that ulcers appear more frequently in male than in female animals, and the ratio is 1:25. The percent representation of these changes is, according to certain investigations, 23.5% in males and 17.6% in females (Curtin et al., 1963). It has also been claimed that the incidence of ulcers is not related to the sex of the animal (Aleksic´, 1987; Guise et al., 1997; Milic´ et al., 1968; Muggenburg et al., 1964; Olivier and Houix, 1969). There is frequent disagreement regarding the influence of the breed of swine on the incidence and frequency of esophagogastric lesions in swine. Gastric ulcers have been established in swine of diVerent breeds. More primitive breeds are more resistant (Lecompte, 1966), and it has been claimed (Aleksic´, 1987; Curtin et al., 1963) that breed has no influence on the appearance or frequency of esophagogastric ulcers. Opinions of researchers are divided regarding the influence of the seasons of the year on the appearance or frequency of ulcers. According to some (Curtin et al., 1963; Hoextra, 1967), they occur most frequently in the winter months, especially in December and January, although there are views that the season has no eVect on the appearance of this disease (Aleksic´, 1987; Sˇenk, 1978).

II. Morphofunctional Features of Swine Stomach The shape of the swine stomach is sack‐like and it is positioned sideways in the abdominal cavity. It has two diVerent ends (the left or cardiac and the right or pyloric), two surfaces (cranial and caudal), and two edges (dorsal and ventral), and the central part––the corpus ventriculi. There are two openings on the stomach—the opening that links it to the esophagus, the ostium cardiacum, and the opening that leads to the small intestine, the ostium pyloricum. The cardia has a circular muscle (m. sphincter cardiae) and the pylorus has the m. sphincter pylori. The left side of the stomach is larger and more rounded, while the right side is smaller and narrower. The cranial surface is slightly extended and leans on the diaphragm and liver––the facies diaphragmatica. The caudal surface of the stomach is curved and leans on the intestines––the facies intestinales. The dorsal edge is concave and is marked as a small curve––the curvatura ventriculi minor, and it spreads between the esophagus and the duodenum. The ventral edge of the stomach, or the ventral curve, is extended, almost semicircular in shape, and larger, so that it is marked as

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the big curve––the curvatura ventriculi major. The stomach is connected to neighboring organs through the esophagus to the diaphragm, to the dorsal abdominal wall, actually to the aorta, through blood vessels, and to the spleen, liver, and duodenum through the duplication of the peritoneum (Sison, 1962). Cutaneous and glandular mucosa of swine, as in most domestic animals, follows one another within this organ, which is why it is called a complex stomach––the ventriculus compositus. The part of the stomach that has cutaneous mucosa and that is located around the entry of the esophagus into the stomach is called the esophageal or prestomach part––the pars esophagica or proventricularis. The other part of the stomach, which is lined with glandular mucosa, is called the glandular or real stomach––the pars glandularis. The border between the two mucosa consists of a fold, and there is also a very visible diVerence in its color. The gaster mucosa of swine has four regions. The initial esophageal part along the line of the big curve covers 3.13 cm, actually, depending on the size of the stomach, from 2.4–5.25 cm. There are no glandular elements in this region, while there is squamous stratified epithelium on the surface. The transition from this part into the cardiac area is marked by the appearance of glands that are spread across 8.5 cm (6.7–11.6). From the beginning of this zone, at a distance of 5.2–9.6 cm, there are bordering, and somewhat further also main cells, which mark the beginning of the fundus area that covers an average of 19.58 cm (14.2–23.8) of the big curve. Further on there is the pylorus, which imperceptibly turns into the duodenum (Petrosjan, 1975). Beginning from the cardia, up until the end of the stomach, the internal surface of this organ is covered with one row of cylindrical or prismatic cells that also coats the gastric foveolas. Numerous granules containing specific mucus have been discovered in the cytoplasm of these cells using cytochemical investigations (Panasjuk et al., 1979). Surface cells of the stomach mucosa make up a very unstable cell population. It has been proven that the entire surface layer is replaced every 3–9 days. This regeneration is secured from immature cells located in the lower part of the crypt and in the neck of the fundic glands. A further characteristic of the superficial epithelium is its uniformity, which is why it is impossible to observe in certain morphological types of cells, on the grounds of which the chain of functional activity could be reconstructed (Panasjuk et al., 1979). The lamina propria of the stomach mucosa, in addition to cardiac and pyloric glands of predominantly mucous character, also contains the main glands in the fundus. The border, chief, mucous, and endocrine cells are located in them. Regarding the numerical ratio of these elements in the fundic glands of the swine stomach, data available so far are very scant, and sometimes even contradictory. While some (Keneth, 1975; Otto and Hugo, 1960) believe that they are equally represented along the entire length of the glandular tubule, others report that individual parietal cells are interspaced

ESOPHAGOGASTRIC LESIONS IN PIGS

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between the primary ones, and that there is a slightly larger number of them in the upper and central third of the glands. According to Petrosjan (1975) parietal cells are not located individually, but in groups, closely adjacent to each other, so that they sometimes fill out the entire lumen of the tubule. The role of parietal cells also includes the secretion of HCl. Since these cells do not have the ability to multiply, their regeneration is secured from immature cells of the glandular necks. The main cells are mostly located in the basal part of the gland. Their function is the synthesis and secretion of pepsinogen (Keneth, 1975). The origin of these cells has not been defined with certainty yet. Mucous cells of the stomach glands secrete mucoproteins that form a net in their physiological concentration. The net presents a viscous elastic gel that continuously lines the entire mucosa of the stomach, functioning like a barrier against numerous harmful agents (Allen et al., 1984; Rokkjaer et al., 1979; Turner et al., 1985). Stanley and associates (1983) have demonstrated that mucins of the swine stomach are a very heterogeneous group according to both size and composition, and that they can be divided into two groups: one with a high content of sulfur and another with a lower content. Mucus glucoproteins have been isolated from the cardiac, fundic, and pyloric parts of the swine stomach. There was more mucin in the cardial and pylorus regions than in the fundus. The protein part of glucoproteins is characterized by a smaller content of threonine and serine in the following declining sequence: cardia, fundus, pylorus. Based on hydrocarbon composition, five populations of mucins have been isolated from the region of the cardia, corpus, and antrum of the gastric mucosa in swine. Using gas chromatography and mass spectrometry, 30 diVerent oligosaccharides have been described, composed of up to six monosaccharide units. One group of oligosaccharides in the central part contains Galb1–3/GalNAca1 and another with a Galb1–3/GalNAcb1–6/ GalNAca1 structure is widely represented, while oligosaccharides with a structure containing Ga1NAcb1–3/GalNAca1 are present in mucins of the cardia and corpus. An oligosaccharide unit composed of GalNAcb1–3/ GalNAcb1–6/GalNAca1 was found in cardia mucin. Gastric mucin of the swine contains large quantities of free fatty acids and cholesterol, as well as some sphingomyelin and phospholipids. As lipids have the ability to collect free radicals from oxygen, they maintain the stability of the mucoprotein viscosity within physiological limits. The main characteristics of the mucus from which their primary protective function is derived are adhesivity, viscosity, and the ability to absorb and neutralize acid. Most of these characteristics are conditioned by the presence of mucoproteins, which are an important component of mucus. The mucin population of the swine stomach is structurally diverse and it is determined as neutral (fucomucin) and more (sulfomucin) or less (sialomucin) acidic using histochemical methods.

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Histochemical investigations of stomach mucins of mammals show that there are diVerences among them, both regarding topography, and also regarding animal species. In dogs, for instance, fuco‐, sialo‐, and sulfomucins have been established in the surface epithelium of the pylorus, while sulfomucins were established in the foveolas of these regions. In humans, fucomucins have been found in the superficial epithelium of the fundus and antrum, and sialomucins in gastric pits of these regions (Keneth, 1975). Histochemical analysis of quantitative–qualitative relations between acid and neutral mucins in the stomach of healthy swine revealed diVerences in the regional distribution. At the cardiac level in the surface and foveolar epithelium there are only acid mucins, while glandular tubules contain exclusively neutral mucins. In the fundus, at the level of the surface and foveolar epithelium, there is a mixture of acid and neutral mucoproteins, and gastric glands contain only neutral ones. In the pylorus, mixtures of acid and neutral mucosubstances are evident at all three levels (Aleksic´, 1987; Aleksic´ and Knezˇevic´, 1989a–c). The swine stomach and intestinal mucosa also contain disseminated individual endocrine cells that lie directly on the basal membrane of the epithelium (Cetin, 1992; Kvetnoy et al., 1997; Solcia et al., 1995b; Zufarov et al., 1978). According to general cytochemical and functional characteristics, they belong to a specific group of diVerent cell types, which together form the so‐called APUD system. A unique hypothesis on the existence of individual cells responsible for production and the secretion of polypeptide hormones was established by Pearse (1960). Investigations of the APUD system and its significance in the pathogenesis of ulcer and other diseases have been continued (Grube, 1976; Grube and Forssmann, 1978; Pearse, 1960; Pearse et al., 1974, 1977). Enteroendocrine cells stained using empirical methods are observed with light microscopy as diVerent morphological forms localized along the basal membrane of the epithelium of the entire gastrointestinal tract . They are most numerous in the pars pylorica and the duodenum. Electron microscopic observations reveal their relatively light cytoplasm, small and wide mitochondria, and very developed microvilli. The most important characteristic of enteroendocrine cells is the morphology of their secretory granules. In addition to cells with polymorphic granules, of large electronic density, there are also cells with oval and round granules. The diVerent appearance of the granules was earlier considered hypothetically as an equivalent to the diVerent functions of endocrine cells, on the basis of which they were classified (Grube and Forssmann, 1978; Kretutzfeldt, 1970). Today, APUD cells are identified on the basis of the type of hormone that they produce (Kvetnoy et al., 1997). So far, G, ECL, EC, D, and A enteroendocrine cells have been established in diVerent regions of the stomach. Each of them has the ability to synthesize a certain polypeptide hormone or biogenic amine.

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Using classical hematoxylin and eosin staining, G cells have been described as ‘‘light’’ and triangular, with a large ovoid nuclei (Solcia et al., 1969), whose topographic distribution depends on the biological species, so that they are most numerous in the mammals examined in the antropyloric mucosa (Bussolati and Canese, 1972; Bussolati and Monga, 1973; Bussolati and Pearse, 1970; Larsson, 1975; Vassallo et al., 1969, 1971). They are also present in substantial numbers in the duodenum of the cat, the dog, and in humans (Solcia et al., 1975). In the mouse, rat, and rabbit, G cells are localized in the basal half of the antropyloric mucosa, while in the cat, dog, and humans, they are located in the central part of the glandular zone of this region (Solcia et al., 1975). Using immunocytochemical analysis (peroxidase–antiperoxidase) in sections of stomachs of healthy swine, it was established that G cells are located mostly along the central zone of the antral mucosa. They are located in the surface epithelium and pyloric glands, individually or in groups, interspersed between other glandular cells. The average number of G cells in the pylorus of healthy swine amounts to 9.27 (Knezˇevic´ et al., 1994). The number of G cells/mm2 was similar in swine with or without esophagogastric ulcer. Investigations of the level of serum gastrin did not reveal significant diVerences between swine with and those without this ulcer (Silva et al., 2002). Today, it is certain that this type of cell secretes gastrin, whose experimental eVect depends on the size of the applied dose. Small doses stimulate secretion of water and electrolytes at the level of the stomach, pancreas, and Brunner glands and the contraction of the cardiac sphincter and the stomach muscle. At the same time, gastrin inhibits the tonus of the sphincter of Oddi and the absorption of water and electrolytes in the ileum. Furthermore, it increases the blood flow through the stomach mucosa, releases histamine, and induces the activity of histidine decarboxylases in the stomach mucosa. Large doses of gastrin have a trophic eVect on cells of the stomach mucosa, as well as a stimulative eVect on the smooth muscles of the intestines, the gallbladder, and the uterus. In humans with a stomach peptic ulcer, the number of G cells is extremely reduced, which points to their role in the complex etiopathogenesis of these diseases (Katic´, 1979). In swine with experimentally induced lesions in the esophagogastric region, it has been proven that the number of G cells is reduced in comparison with their number in healthy animals (Knezˇevic´ et al., 1994). Ultrastructural investigations have resulted in the identification of two (Bordi et al., 1995) and three (Solcia et al., 1995a; Valverde et al., 1993) types of endocrine cells, which have been marked, depending on their presence in certain parts of the gastrointestinal tract, as stomach, intestinal, and duodenal. The stomach type of endocrine cells is elongated in shape with small rod‐ like and pear‐shaped granules, which are set parallel to the basal membrane and are of an open type (Katic´, 1979). In humans, they are localized in the pyloric glands and immediately adjacent to the lamina muscularis of the mucosa. They

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are uniformly wedge‐shaped with a narrow cytoplasmatic edge. Their number is most often reduced in humans with a stomach ulcer (Katic´, 1979). Intestinal endocrine cells are large, pyramidal, or bottle‐shaped, with a greater quantity of granules that are somewhat larger localized in all parts of the intestine (Sasagawa et al., 1974). In the stomach antrum mucosa of humans with a stomach ulcer, their number is significantly increased with the almost complete disappearance of G cells (Katic´, 1979). The third duodenal type of endocrine cells contains large irregular (ovoid or angular) granules, pyramidal or bottle‐ shaped. Using cytochemical methods, 5‐hydroxytryptamine (5‐HT) was discovered in very small quantities in granules of endocrine cells. It is believed that this biogenic amine has a role in the control of stomach secretion by inhibiting the secretion of acidogen (Wise, 1974). Its stimulative eVect on mucin secretion and its eVect on the smooth muscles and tonus of blood vessels are also known. Sections of fundic mucosa of stomachs of healthy swine reveal enteroendocrine cells of diVerent morphology, along the entire length of the gastric glands. The most numerous shapes of these cells are dark brown to black stained granules that completely mask the nucleus, the largest in size, round‐ shaped, with marginally distributed dark stained granules, with a centrally placed nucleus. Spindle‐shaped, slightly less stained than the previous cells, which are dominant according to their presence are elliptical with extremely dark brown stained granules. All endocrine cells are located between other glandular elements and are mostly placed along the basal membrane. Most of them are concentrated at the basal portion and in the body of the gastric glandules. Histochemical analysis of sections of the pyloric region of stomachs of healthy swine shows endocrine cellular elements deeply dispersed in the lower and central third of the pyloric glands. Cells of round and roundish shape are predominant, with clearly expressed granules in the cytoplasm, filling out the contours of the cell membrane, sometimes completely giving them the appearance of homogeneous black cells. Most often, the number of granules is smaller and they are lightly stained, making the cell appear transparent. In some cases, the granules are concentrated at the poles, similar in appearance to polar caps. Stereometric processing showed an average of 25.85 cells/mm2 of fundus, and 38.28 endocrine cells in the pylorus (Grimelius positive). A significantly greater number of endocrine cells was discovered in the pylorus than in the fundus ( p < 0.001) (Aleksic´, 1987; Aleksic´ et al., 1993; Knezˇevic´ et al., 1994). Stereometric analysis of a series of sections of the stomach mucosa of swine with spontaneous ulcers showed an average of 18.69 Grimelius‐positive cells/mm2 of fundus, and 25.85 on the pylorus. A significantly smaller number of endocrine cells was also established in the fundus ( p < 0.005) and

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in the pylorus ( p < 0.001) in the stomachs of these swine in comparison with controls (Aleksic´, 1987; Aleksic´ et al., 1993; Knezˇevic´ et al., 1994). Stereometric analysis of a series of sections of the stomach mucosa of swine with experimentally induced ulcers showed 30.47 endocrine cells/mm2 of fundus, and 27.04 cells in the pylorus. No statistically significant diVerences were established in the number of these cell elements in the fundus of this group ( p < 0.05) versus the control. Significance was established in the pylorus ( p < 0.001) (Aleksic´, 1987; Aleksic´ et al., 1993). The precise role of hormones in the regulation of glandular mobility has not been completely elucidated yet. It seems that gastrin, which is secreted by pylorus cells, increases the motility of the stomach. Cholecystokinin, secretin, and gastric inhibitory peptide suppress gastric motility. Gastric secretions are produced by gastric glands and epithelial cells of the stomach mucosa. It is composed of water, Kþ, Naþ, Mg2þ, Hþ, Cl , HPO42 , SO42 , pepsinogen, labferment, lipase, protective mucins, and the internal factor. When gastric glands are maximally stimulated they secrete a solution of HCl of pH 1 into the lumen. Hydrogen and chloride ions are secreted by parietal cells through diVerent cellular mechanisms. Hydrogen is secreted through primary active transport with the help of the Hþ/Kþ‐ATPase pump, which is located on the luminal side of parietal cells. This enzyme replaces a hydrogen ion with one Kþ ion by ejecting one hydrogen for every potassium, which returns from the stomach lumen to the cytoplasm of parietal cells. As Kþ ions are accumulated in the cell by a passive mechanism they return to the stomach lumen, which is known as potassium recirculation. Chloride ions originating from blood also passively enter the stomach lumen. For each hydrogen ion that is secreted into the stomach lumen, one bicarbonate ion leaves the cell and returns into the circulation. Chloride ions at the same time return to parietal cells through an antiport mechanism. Carbon acid originates from enzyme activities of carbonic anhydrase, which is present in a high concentration in the gastric mucosa. As in other cells, the Na/K‐ATPase pump is active in the basal part of parietal cells (Cuningham, 1992). Pepsin is usually marked as one enzyme, even though it is in fact a group of proteases that is secreted by gastric glands. They are formed in the main cells in the form of the proenzyme pepsinogen. Pepsinogens are deposited in granules of the main cells until secreted into the stomach lumen, where they are activated under the activity of hydrogen ions. The presence of inactive proenzymes is necessary because active enzymes could destroy the cell that synthesized them. Gastric gland secretion is stimulated by the intake of food, as well as the presence of undigested content in the stomach. When the animal begins to eat, parasympathetic vagus impulses stimulate cells of the intramural gastrointestinal nervous system, and acetylcholine is released near parietal and G cells. These cells have, on their surface, acetylcholine

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receptors and respond by secreting gastrin and HCl. Through blood, gastrin (the endocrine eVect) reaches parietal cells, which also have gastrin receptors. A combined eVect of gastrin and acetylcholine on parietal cells leads to the secretion of large quantities of HCl. Monitoring of the level of plasmatic gastrin and pepsinogen in swine with hyperplasia of the epithelium and ulcerations of the pars esophagica did not reveal any diVerences in comparison with healthy swine (Bunn et al., 1981). However, in cases with parakeratosis, erosions and ulcerations in the esophageal region show increased concentrations of pepsinogen in serum (Nappert et al., 1990). The role of histamine in HCl secretion is still not suYciently clear. It is released by mast cells of the stomach mucosa under the eVects of gastrin and acetylcholine. Parietal cells also contain Hl and H2 receptors, which means that their secretion is stimulated by three mediators––acetylcholine, gastrin, and histamine. The secretion of pepsinogen seems to be under the same regulatory eVects as the secretion of HCl.

III. Esophagogastric Ulcer in Swine A. Etiology and Pathogenesis The most numerous investigations pertain to the role of food and its individual components in the development of esophagogastric ulcers. It was mostly attempted under experimental conditions to provoke an ulcer using certain ingredients of a fodder mix, or to determine which feed component prevents or eases the appearance of ulcerous processes. Some of the first papers published in this area concluded that food can have an eVect on the appearance of an ulcer (Fugate et al., 1965; Mahan et al., 1966a; Nuner et al., 1966; Perry et al., 1962; Resse et al., 1966). Data presented later also concur with these findings, and the causes should not be sought in the composition of the food itself, but rather in the form in which it is administered, especially regarding the size of its granules (Baustad and Nafstad, 1969; Dirrsen, 1964; Ehrensperger et al., 1976; Fugate et al., 1965; Lengnick, 1972; Mahan et al., 1966b; Mastronardi, 1964; Perry et al., 1962; Pococov et al., 1968; Reimann et al., 1967). A diet of finely ground and floury feed with large numbers of tiny granules, as well as with feed in pellet form, favors the appearance of keratinization of the esophageal mucosa and the creation of erosions. According to the latest research in swine with frequent keratinization of the mucosa and ulcers in the esophagogastric part, 90% of the feed, regardless of how the ration is composed, has a floury structure with a radius of the granules of less than 1.5 mm (Larenaudie et al., 1966; Lengnick, 1972; Wondra et al., 1995). On farms where medium‐sized granules of 1.5 mm and

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larger account for at least 3% of the feed, and finely ground granules for 96%, changes in the cutaneous mucosa of the stomach are the most frequent and of the gravest form. However, if the feed contains a larger part of rougher granules, changes in the esophageal part of the stomach have been observed less frequently. The size of the granule determines its disintegration in the stomach. If the food fails to contain a suYcient number of rough and coarse fragments there is no natural wasting and renewal of the epithelium of the cutaneous mucosa of the proventricular part of the stomach. Furthermore, food of very fine structure passes the gaster more quickly so that there are no mechanical factors responsible for the shedding and renewing of the epithelium. Perhaps this could explain the excessive keratinization of the stomach mucosa, and primarily of its esophageal part (Elbers et al., 1995; Lengnick, 1972). The disorders in the keratinization could be a consequence of long‐term acidosis connected to the chemical processes of digestion under the influence of stomach juices and microbiotic activities. Disrupted keratinization, as it is known, does not necessarily lead to the appearance of an ulcer, even though most researchers consider it as its initial stage. Microbiological investigations of material from the ulcer have shown that there are often fungi of the Candida species present, which has led to the conclusion that they could be the possible cause of the appearance of an ulcer (Curtin et al., 1963; Ehrensperger et al., 1976; GriYng, 1963; Hunziker and Nicolet, 1968b). Experimental works have proven that Candida albicans presents as a normal member of the stomach flora of swine (GriYng, 1963; Kadel et al., 1969; Smith, 1976), as well as that the injection of its pure culture in the course of 49 days did not reveal the appearance of any lesions in the esophagogastric region (Stenham et al., 1967). Even though one study discovered the presence of fungi of the genus Candida in the parakeratotic layer in ulcerous lesions and detritus in peptic necrosis, they have not been given any importance in the morphogenesis of the ulcer (Sˇenk, 1978). Colonization by the spiral bacteria Helicobacter type 1 or Gastrospirilum suis was established in swine with spontaneous peptic ulcerations in the pars esophagica (Mall et al., 2004; Szeredi et al., 2005). Even though these microorganisms do not invade pars esophagica cells and do not perform toxic destruction of the cellular elements, a role in the pathogenesis of lesions has been attributed to them. These microorganisms have been established in 100% of examined swine that had a developed ulcer and in 90% of swine with preulcerous lesions (hyperkeratosis) (Barbosa et al., 1995; Krakowka et al., 1995, 2005a,b; Querioz et al., 1996; Suarez et al., 1997). One possibility for the ulcerogenic eVect of bacteria could be their ability to create lower fatty acids. Nondissociated lower fatty acids quickly pass through the outer barrier of the stomach mucosa and increase the acidity of the stomach mucosa. Cellular acidification inhibits the Na pump and osmoregulation, which leads to cellular edema and necrosis (Argenzio and Eisemann, 1996).

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The eVect of certain vitamins on the etiopathogenesis of lesions in the esophageal region has been examined. Thus, it has been reported for vitamins A and D that they have a protective role (Larenaudie et al., 1966), and for vitamins E and K that, when added to food or applied intramuscularly, they prevent the development of erosions in the stomach mucosa (Coates et al., 1998; Hannan and Nyhan, 1962). The latest investigations have shown that the administration of melatonin in feed (5 mg/kg feed) significantly reduces the frequency of the incidence of esophagogastric ulcer in swine (Bubenik et al., 1998). An especially interesting group of investigations, which deal with the etiopathogenesis of this disease, involve the eVects of diVerent technological procedures in the industrial maintenance of swine. This deals particularly with the type of maintenance conditions, the accommodation facilities for the animals, their treatment, and the like. It has been emphasized that a stomach ulcer develops in swine, as the ulcer in humans, under the eVect of stress. In contemporary breeding conditions, swine are exposed to numerous nonspecific irritants, which causes them to feel anxiety, tension, fear, pain, and so on (Bencˇevic´, 1972; Hunziker and Nicolet, 1968a; Kowalczyk and Muggenburg, 1963; Milic´ et al., 1968; Sˇabec et al., 1971; Tournut and Lebie, 1970). This acts as a stress factor of a psychosomatic and physical nature, demanding the occasional or permanent adapting of the animal to the given conditions of the environment and its frequent changes. Esophagogastric ulcers should therefore be classified in the group of diseases whose causes are a consequence of a general syndrome of adapting. More recent literature warns against an entire series of possible nonspecific factors for which it has been proven, or it is believed, that they considerably increase the incidence of ulcers. The observations deal with stress situations caused by limited living conditions (Curtin et al., 1963; Handlin et al., 1972; Kowalczyk and Muggenburg, 1963; Larenaudie et al., 1966; Muggenburg et al., 1971; Resse et al., 1966). Changes in temperature and atmospheric conditions of the environment (Curtin et al., 1963), transportation, the stay in the depot prior to slaughter, the mixing of animals that are not familiar with each other, and a new unknown environment are also dealt with (Hoextra and Grummer, 1967; Kowalczyk, 1970; Resse et al., 1966; Tournut et al., 1966). Especially prominent are the experimental works by researchers from France, who have observed significant changes in the digestive tract of piglets forcibly immobilized with the help of a special device (Labie et al., 1966; Le Bars and Tournut, 1962; Tournut et al., 1966). Changes of the ulcer type have been established in the mucosa of their stomachs. In swine with esophagogastric ulcers, neuroendocrine regulation has been disrupted in the sense that there is a reduced secretion of the thyreotropic hormone of the adenohypophysis, triiodothyronine and thyroxine of the thyroid gland, and increased secretion of cortisone. Since there is an

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increased secretion of corticotropin at the expense of thyreotropin under conditions of stress, and they are both under the control of the hypothalamus, the described changes in endocrine correlation could be interpreted as a contribution to evidence that neurostress is very important in the etiopathogenesis of ulcer disease (Simov, 1977). To understand the etiology of the stomach ulcer in swine, the significance of excess acidity of stomach juice was investigated (Huber and Wallin, 1967; Muggenburg et al., 1966b). Imitating histamine secretion in stress conditions, it was applied in a dose of 2.5 mg/kg body mass of swine, inducing great ulcers in the esophageal part of the stomach (Kokue et al., 1981; Muggenburg et al., 1966b). The same eVect was obtained with the intramuscular application of reserpine in quantities of at least 0.055 mg/kg body mass, during 15, or 14 and 21 days (Aleksic´, 1987; Aleksic´ and Knezˇevic´, 1989a; Muggenburg et al., 1966a), or with the parallel administration of histamine and reserpine (Muggenburg et al., 1967). It was shown that histamine and reserpine considerably increase the secretion of HCl, thus lowering the pH of the stomach content. Throughout this, pepsin activity is not altered, or it is increased as well. It is believed that the ulcerogenic eVect of reserpine is mostly based on the lesions that it causes in the diencephalon (Mastronardi, 1964), which in yet another way confirms the assumption about the role of neurovegetative disorders in the etiopathogenesis of the ulcer (Hunziker and Nicolet, 1968b; Simov, 1977). In addition to histamine and reserpine, sodium salicylate also causes lesions in the pars esophagica (Petrosjan et al., 1976). Prednisolone, as well as the binding of the pylorus in experimental conditions, also leads to the appearance of an ulcer (Nelson, 1966). There is irrefutable evidence that the decreased secretion of stomach mucus and changes in its composition have a role in the occurrence of esophagogastric ulcers in swine. A histochemical analysis of the distribution and qualitative–quantitative relations of mucin in the normal gastric mucus of humans has proven the increased presence of neutral mucins in the surface epithelium of the fundic (corpus) mucosa and the antrum, in the upper half of the foveolar epithelium of the same region, as well as in the pyloric glands, while a smaller presence was observed in the lower half of the foveolas, and somewhat higher quantities in the neck part of the corpus glands. Gaster mucosa in humans with a stomach ulcer was found to contain a smaller reduction of fucomucin in 60% of patients, while mucins in traces were present in 7% of the studied patients (Katic´, 1979). The question of the pathways for the occurrence of increased viscosity of mucin in the swine stomach has not been fully explained yet because of the numerous contradictory data that have been obtained. There is no doubt that the mucin viscosity is altered with the reduction of the pH value of the stomach juices. It increases up to 100 times, which indicates the physiological importance of the changes in the rheological characteristics of mucus.

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This is one of the ways in which mucins protect the stomach mucosa when pH values are low. It remains an outstanding issue whether the formation of extremely large aggregates of mucus glycoproteins at pH values that go down to 2 or 1 is a result of the merging of polypeptide components of proteoglucan, of a molecular mass of 2.54 106 and 1.5 106 Da (Bennett and McLean, 1985; Bhaskar et al., 1991), or whether it is a matter of carbohydrate reactions that cause aggregation (Sellers and Allen, 1989). A binding peptide is also probably involved in this process, which is a glycopeptide. This protein has been found in mucins of the gastrointestinal tract, including the salivary glands, the stomach, intestine, and colon. Its molecular mass is 118 kDa, and it enables mucin polymerization by forming disulfide bridges between mucin glycoprotein subunits (Roberton et al., 1989). Polymerized gastric mucins cover the stomach mucosa, protecting it from the harmful eVects of acid, proteases, and in particular, pepsin and bile salts. An important common characteristic of mucins is the ability to bind lipids. Bound lipids collect free radicals of oxygen. Gastric mucins of swine contain large quantities of free fatty acids and cholesterol, as well as some sphingomyelin and phospholipids. The iron/ascorbate system creates free radicals of oxygen, which reduce the specific viscosity of mucins by more than 50% (Grisham et al., 1987). Excessive production of oxygen radicals can be inhibited by catalases, deferoxamine, and mannitol, while superoxide dismutase has no eVect. In the event the mucins are purified, actually freed of the fatty acids, the oxygen metabolites have no eVect, which shows that bound lipids protect the surface of the stomach mucosa from depolymerization of native mucins (Fouad et al., 1993; Gong et al., 1990). In swine with experimentally induced esophagogastric ulcerations, there was a higher protein content in the mucus in comparison with healthy swine, and a reduced amount of N‐acetylgalactosamine and fucosis (Mall et al., 1997). In the appearance of peptic ulcerations, it is possible that changes in the regenerative ability of mucosa cells in the stomach and intestines can play a certain role. Here, the primary reference is to the disorders in the control of proliferation, diVerentiation, and migration of gastric epithelial cells. These disorders can be a result of genetic factors or factors of the environment. Among the local factors that can be considered are the diet, microcirculation, and growth factors (Kawai and Rokutan, 1995; Sˇabec et al., 1967). The present understanding of the etiopathogenesis of ulcers is based on the fact that the essential reason for the appearance of lesions is actually the disturbed relations between so‐called aggressive and defensive factors of the stomach mucosa. The aggressive factors include stomach acid and proteolytic ferments, while mucins and the great regenerative power of the surface epithelium present defensive factors (Curtin, 1966; Palavicin et al., 1971). Histochemical analyses of stomachs of swine with spontaneous esophagogastric ulcers show a considerably reduced total amount of mucins,

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even though no diVerences have been established in the qualitative distribution of acid and neutral mucoproteins (Aleksic´, 1987; Aleksic´ and Knezˇevic´, 1989c). In stomachs of swine with experimentally induced lesions in the esophageal region (reserpine), the amount of total mucins is greater than in the stomachs of healthy animals. The quantity of established mucins is also greater in comparison with the stomachs of swine with spontaneously developed ulcers. Even though the total amount of mucins is increased, neutral mucins were not established at the level of the foveolar epithelium of the fundus (Aleksic´, 1987; Aleksic´ and Knezˇevic´, 1989b).

B. Pathomorphological Findings 1. Macroscopic Findings Since the pathomorphological picture of possible changes in the pars proventricularis in the presence of an ulcer is not unique, it follows that the reviewed literature dealing with this matter provides very diverse data. Nevertheless, most studies divide all alterations into three groups: acute erosions, subacute ulcers, and chronic ulcers (Kretutzfeldt, 1970; Sˇenk and Sˇabec, 1965). Due to the desquamation of the epithelium, the areals of papilla propria remain bare, and their conflation results in the occurrence of acute erosions. Their size varies, and ranges from those hardly noticeable, 0.2 cm in diameter, to the largest ones, 2 cm in diameter. They are irregular in shape and often elongated or egg‐shaped. Their base is covered with pseudomembranes, dark brown in color from ingredients from the blood, or reddish due to local hyperemia. They are most often surrounded by a yellow‐gray rough hyperkeratotic surface (Thoonen and Hoorens, 1963a) (Fig. 1). Subacute ulcers are flat, larger, and have deeper defects in the esophagogastric region from erosions, from 0.5–4 cm in diameter. They are mostly inflamed and oval or crescent shaped in appearance. Their bottom is covered with necrotic sediments under which is a layer of edematous granulation tissue, light pink in color (Thoonen and Hoorens, 1963b). Chronic ulcers are deep defects in the mucosa, clearly defined from the surrounding unchanged tissue with a sharp edge that rises above the ulcer crater. They are most often round or irregularly ovoid in shape and of diVerent dimensions (Fedorov et al., 1977; Petrosjan, 1975). Their size depends on the age of the animal. In younger animals, it reaches the dimensions of a child’s palm (4–5 4–6 cm); in older animals they can be up to 8 9 cm (Sˇenk and Sˇabec, 1965). They often cover the entire esophageal area. Their base is dark gray in color and in folds.

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FIG. 1 Gaster of pig, hyperkeratosis (h).

Based on examinations of large numbers of pigs with esophagogastric ulcers who died spontaneously, it can be said that they basically have the same macroscopic and microscopic appearance. There are usually round or oval defects in the mucosa that penetrate at least into the submucosa, usually to the muscularis, and sometimes even deeper. They are clearly separated from the other, unchanged, parts of the mucosa, and have sharp or slightly rounded edges that are higher than the ulcer crater. The base of the ulcer is uneven, and it is covered with pseudomembranes or coagulum residue of dark brown color. They are from 4 6 cm–8 10 cm in diameter, sometimes covering the entire area of the cutaneous mucus. The depth of the ulcer diVers from case to case, and ranges within the limits of 3–6 mm. Sometimes, the ulcer crater penetrates the stomach wall, leading to localized or generalized peritonitis, or perforation of the neighboring tissue structure, such as the omentum, liver, or pancreas (Aleksic´, 1987) (Fig. 2). Under experimental conditions, intramuscular application of reserpine in quantities of 0.055 mg/kg body mass for 14 days caused lesions in the esophagogastric mucus in swine. In a number of cases, a surface defect was observed, localized in the central part of the cutaneous region. One was of irregular roundish shape, with dimensions of 4 5 mm, about 2 mm deep, with a bright pink base and almost invisible borders that limit it from the unchanged mucosa. In another case, a somewhat larger defect was discovered, about 8 mm long and 2 mm deep, with a rough surface on the base that was light pink in color. Swine to which administration of reserpine was continued until day 21 showed dark yellow warty deposits in the esophageal region––hyperkeratosis, diVusely distributed along the entire surface of

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FIG. 2 Gaster of pig, esophagogastric ulcer.

the cutaneous mucosa, making it similar in appearance to the bark of an oak tree. Between the hyperkeratotic deposits there was discrete damage to the mucosa, bright red in color and 3–6 mm in length (Aleksic´, 1987). 2. Microscopic Findings Investigations of histological changes in the pars esophagica have been the subject of numerous studies, starting from the very first descriptions of esophagogastric ulcer to the present day. The large number of data from the literature in this area are at the same time very heterogenic regarding the systematization of the observed changes. Nevertheless, most studies indicate that three basic groups of changes can be described, depending on the nature of the alteration in the esophageal region: (1) preulcerous‐ parakeratotic keratinization of the mucosa, (2) erosive‐ulcerous lesions, and (3) postulcerous and residual alterations (Aleksic´, 1987; Ehrensperger, 1974; Ha¨nichen, 1975; Penny et al., 1972; Petrosjan et al., 1976; Ristoski, 1999; Rothenbacher, 1965; Ryaszkowaki and Gambara, 1976; Sˇenk, 1969; Sˇenk and Sˇabec, 1967; Thoonen and Hoorens, 1963). In more recent times, certain researchers have given more detailed descriptions of these changes in their papers, depending on quantitative–qualitative alterations in the mucosa of the proventricular part. Within preulcerous‐ prekeratotic changes, two types are evident, depending on the degree of damage. The first type includes cases in which the stratified squamous epithelium is of normal thickness and without signs of proliferation, but with the simultaneous appearance of a thin layer on the surface––keratinization with

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18

parakeratosis. The other type covers changes that are reflected in a thickening of the stratified epithelium at the expense of multiplication of cells of the stratum spinosum (acanthosis) with hyperkeratosis and parakeratosis on the surface. Within this type, and based on the degree of keratinization of the stratified squamous epithelium, the following is prominent: (1) keratinization of a smaller degree––moderate hyperplasia of the epithelium (the tips of the papillary shoots reach the chromophobic layer of epithelial cells); (2) keratinization of a higher degree––intensive hyperplasia of the epithelium with stronger keratinization on the surface (the stratified squamous epithelium is thickened and partly shedding; the papillary layer of the propria reaches deep into the epithelium); there is a thick dense layer of squamous keratinized cells with a nucleus on the surface––parakeratosis; (3) extreme hyperplasia of the epithelium with intensive keratinization and the appearance of microerosions (Fig. 3). This degree presents a transition between preulcerous and erosive‐ulcerous changes. Alterations in the epithelium are similar as in the previous two degrees, and they diVer from these in that the surface of the hyperkeratotic layer shows keratotic processes, uncovering the papillary bodies and causing the appearance of microlesions (Sˇenk, 1978). Pathological alterations of the stratified squamous epithelium of the pars proventricularis have been described as atypical hyperkeratosis (Kowalczyk, 1969), parakeratosis, pseudokeratosis (Bencˇevic´, 1972), or dyskeratosis (Lengnick, 1972). Furthermore, ballooning degeneration of cells of the stratum spinosum has also been described, which, together with dyskeratosis,

FIG. 3

Gaster of pig, pars esophagica, huge hyperkeratosis deposits. H&E, 200.

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leads to a thickening of the cutaneous mucosa, making it very hard and yellow‐brown in color. Histological examinations of the region of the stomach with spontaneously developed ulcers showed identical changes in all cases. The preserved cutaneous mucosa shows thick nonstructural homogeneous hyperkeratotic sediments. Although rarely, groups of vacuolized cells of the stratum spinosum can be seen in this mass, giving it the appearance of cartilaginous tissue. Thorny shoots of the papillary bodies are placed deep inside the propria, sometimes even reaching the submucosa. In places where there are breaks in the continuity of the hyperkeratotic layer, shallower or deeper defects can be seen, which always cross the lamina muscularis of the mucosa, shaped like a volcanic crater whose edges go down to the base. In certain cases, the base and edges of such defects are covered by a layer of necrotized tissue under which a reactive inflammation is observed. In closer or further proximity of the ulcus, mature connective tissue is regularly observed, permeated with a tiny‐cellular infiltrate and clearly diVerentiated fatty tissue. The walls of the blood vessels in the zone of the ulcerous defect, as in the other parts of the stomach wall, are thickened and frayed. It is especially diYcult to observe them in the area of the scar connective tissue when their contours merge with the environment without any clear borders. The lumen of such altered blood vessels is reduced as a result of obliteration. In addition, blood vessels with thrombs in organization can also be seen (Aleksic´, 1987) (Fig. 4). Under experimental conditions, following intramuscular application of reserpine in quantities of 0.055 mg/kg body mass over a period of 14 days,

FIG. 4 Gaster of pig, erosion with secondary inflammatory reaction (microabscess). H&E, 200.

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intensive proliferation of papillary bodies of the propria is observed, with spreading to the lamina muscularis of the mucosa. The surface of the epithelium shows a hyperkeratotic layer of diVerent thickness, which is so reduced due to keratolytic processes that the papillary shoots of the propria are completely bare––microulcerations. Sites of deeper eVects are characterized by the absence of tissue of the papillary body. The base of such shallower or deeper defects formed in this way consists of a partially narrow necrotic zone under which there is connective tissue rich in tiny roundish cells with very little connective tissue, which can be seen especially clearly in sections stained with selective methods. The propria of the mucosa around the defect, as well as the submucosa, show inflammable cellular infiltrates of diVuse or focal character. Thus formed cellular infiltrates are also often observed in the starting part of the cardiac zone of the stomach, especially along the very edge of the defect. Blood vessels, as a rule, have thickened walls and are hyperemic (Aleksic´, 1987). In one study, immunohistochemical staining with Ki67 (clone MIBI) and AgNOR protein silver staining were used to evaluate, by means of image analysis, cell proliferation in normal and parakeratotic (parakeratotic hyperkeratosis) epithelia of the pars esophagea. Apoptotic activity was also assessed with the TUNEL assay and compared with cell proliferative parameters. Early lesions of the pars esophagea were characterized by a significant increase in epithelial proliferative activity, while there was no diVerence in apoptotic activity between normal and parakeratotic epithelia (Preziosi et al., 2000). Histopathological examinations of erosions and ulcerations accompanied by hyperkeratotic changes have led to the conclusion that erosions occur directly from the hyperkeratotic changes in the cutaneous mucosa. The latest investigations indicate that the epithelium of the pars esophagica of the swine stomach is more sensitive to irritating eVects of acid stomach content because of the changes in keratin expression. The keratin pairs K4/K13 are present both in normal and in damaged epithelium and their expression in both states is the same. K4 and K13 are expressed in all suprabasal cells, and K5 and K14 only in basal and epibasal cells. K6 is a significant marker of epithelial proliferation and its expression is increased due to hyperkeratosis. Intermediary keratin filaments indicate that epithelial proliferation, which leads to visible hyperkeratosis, is the fundamental element in gastric ulcers in swine (Ristoski et al., 2001; Roels et al., 1997) (Fig. 5). Even though hyperkeratosis is definitely considered a preulcerous lesion, the factors that cause it are still unknown. Activities by aggressive factors of the stomach juice (pepsinogen, HCl) lead to the destruction of the keratinized layer of the epithelium of the pars esophagica, uncovering the tips of the papilla and the upper layers of the epithelium. These tips are unprotected from mechanical and chemical eVects of the stomach content, which causes

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FIG. 5 Gaster of pig, pars esophagica, keratin’s pattern in hyperkeratosis, DP‐anticytokeratin, 100.

tissue reactions among which hyperemia and papillary corpus edema dominate. Consequently, papillae swell even more, becoming more exposed to the eVects of the aggressive factors that cause surface necrosis. This is, at the beginning, limited only to the tips of the papilla, but later penetrate deeper into the tissue. In that way, microscopically visible erosions, microerosions, are formed in the spaces between two papillary tips. Peptic necrosis spreads further, covering the denuded propria, the remnants of the denuded papillary bodies, which increases the erosion and makes it macroscopically visible. These initial changes most often begin on the ventral edge of the pars proventricularis, as well as in the vicinity of the orificium esophagus. At the surface of this defect is a narrow zone of necrosis under which the tissue of the propria is hyperemic, edematous, and richly infiltrated with leukocytes. On the blood vessels of the propria and the submucosa, there are no changes other than dilatation (Bisson, 1967; Sˇenk and Sˇabec, 1965). The ulcer develops with the penetration of the erosive processes into the muscularis of the mucosa and the submucosis. The process begins with the disintegration of the muscle fibers of the muscularis mucosa as a logical consequence of edemic dissociation or direct necrosis, which moves from the surface into the depth (Sˇenk, 1978). Due to the intensive hyperemia and the edema of the submucosis, the tissue swells and the ulcers cannot be observed macroscopically as defects in this phase of their genesis, because they lie at the level of the mucosa of the esophageal part. In edematous tissue, in addition to serous fluid, there are also many fibrin fibers, polymorphonuclears, and local histiocytes. Numerous capillaries are dilated and

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thrombosed (Aleksic´, 1987; Fedorov et al., 1977; Kowalczyk, 1969; Sˇenk, 1978). In the arteries of the submucosa and muscularis, edema intimae and tunicae of the elasticae internae were observed, as well as vacuolization of endothelial cells (Embaye et al., 1990; Hunziker and Nicolet, 1968a). In the next phase of the genesis of the ulcer there is the swelling of the granulation tissue in the propria and parts of the submucosa, which makes a morphological transition from acute to chronic ulcers. Granulation tissue spreads to the intermusculary connective tissue of the tunicae muscularis, making the intermuscular septa thicker. At the beginning, the ulcer is irregular and crescent shaped, and it later takes on the shape of the letter U, or circularly covers the entire esophageal area. Sometimes, the ulcerous changes are limited not only to the pars proventricularis, but also penetrate into the neighboring glandular mucosa. Not rarely, in such cases necrosis covers even the larger blood vessels, which causes extensive bleeding, resulting even in a lethal outcome. On the surface of the chronic ulcers, there is often a wide layer of fibrinoid peptic necrosis, under which a leukocyte demarcation line is formed. In some cases, there is no necrosis, and there is only granulation tissue on the surface, lying on a solid connective‐scar basis. The outcome of residual and postulcerous conditions depends on the character and the dimensions of the previously existing defects. Surface erosions are completely reepithelized, without signs of cicatrization. Focal ulcers heal with a small scar, which somewhat alters the appearance of the esophageal region due to retraction. Ulcers that are spread over the entire surface of the esophagogastric region, or cover its greater part, heal but leave a completely changed normal relief of that part of the stomach. The deeper the ulcer has penetrated, the more scar tissue prevents the closing of the edges of the former crater. In such cases, the retracted remainder of the ulcer stays, lying immediately along the cardia, causing stenosis of its opening with resulting hypertrophy of the muscles in the esophageal wall (Dvornik and Teleonov, 1976; Sˇenk, 1978).

C. Clinical Picture and Differential Diagnosis The clinical picture that accompanies esophagogastric ulcer correlates with the stage of development and the intensity of the pathomorphological changes in the pars esophagica. In peracute cases, due to the extremely rapid development of ulcerous changes, there are no visible disorders in the general health of the diseased animal. Due to the massive gastrorrhagias, the swine die suddenly, or are in a state of collapse for a brief period of time. The extreme paleness of the mucosa and the skin of the carcasses indicates that esophagogastric ulcers are the most probable cause of death.

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In acute cases of the disease, the skin and mucosa are extremely pale over a certain period prior to death because of the permanent or occasional bleeding into the stomach lumen. The body temperature is within physiological limits. Certain animals gnash their teeth, and because of the pain in their stomach, they take less food, or occasionally refuse to take it. They withdraw to the corners of the facility, move listlessly, and usually lie down. In some cases vomitus can be observed. The vomited stomach contents are dark due to the presence of blood, and similar to ground coVee deposits. Also due to the presence of blood, their feces is also dark, almost the color of tar (melena) (Mackin et al., 1997; Trobo et al., 1994). The clinical picture of the disease in subacute and chronic cases is similar to the course of the acute cases, but the symptoms are somewhat less intense because of the longer course of the disease. The animals are anemic, they take less food, and gradually lose weight. Melena is occasionally observed. Often, the only indication of the presence of an ulcer is the occasional appearance of a hard stool as a result of the obstipation and melena. The course of the disease can be quite long. In many cases, the symptoms of the disease can be covered up by the more strongly expressed symptoms of some other disease (colibacillosis, dysentery, parasitic invasion, and others). Hematological changes depend on the duration of the course of the disease and the intensity of the bleeding. In almost all cases there is oligocythemic and hypochromic anemia. Clinical symptoms similar to those that accompany esophagogastric ulcer are also encountered in cases of the appearance of dysentery, salmonellosis, transmissive––gastroenteritis, intestinal adenomatosis, coccidiosis, ileus, and others. Bacterial and viral infections are most often manifested with a high body temperature and the outbreak of the illness in large numbers of animals simultaneously, contrary to esophagogastric ulcer, where the body temperature is within physiological limits and that occurs sporadically. Unless esophagogastric ulcer is timely diagnosed and unless the necessary therapy is administered, the disease has a lethal outcome following a shorter or a longer time period.

D. Therapy and Prophylaxis Treatment of the initial stage of the ulcerous disease is often lacking because it is practically impossible to set a diagnosis at this stage of the disease. The administration of medicines that (step up the process) stimulate blood coagulation (hemostatics) has not produced any satisfactory results so far. In certain cases, antacid preparations are applied successfully (aluminium hydroxide or magnesium silicate), which are added to food in quantities of 2–3%. Since treatment is in all cases symptomatic, the administration of

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infusion solutions (5% glucose solution––ionlactate and others) or preparations based on iron, vitamin B complexes, and tranquilizers is recommended. The peroral administration of astringents (acidum tannicum, bismuthum subnitricum), as well as preparations that protect the mucosa (mucosin), is indicated. During treatment, the animals should be isolated into separate boxes and protected from stressful eVects. Since physical and chemical characteristics of food present one of the most important factors that cause morphological changes in the stomach mucosa, special attention during prophylaxis must be paid to the size of the feed particles, which should not be smaller than 3 mm. Furthermore, the food must be kept in conditions that will not permit the growth of fungi, thus preventing the formation of unsaturated fatty acids. The enrichment of fodder mixes with vitamin E (18 mg/kg feed with or without added selenium) yields modest results in the prevention of this disease. The application of vitamin U (20 g/100 kg feed––0.001%) has an anti‐inflammatory and analgetic eVect, it protects the mucosa, and it secures the speedier regeneration of the damaged epithelium. When copper is used as a feed additive to stimulate growth, the application of zinc carbonate, in quantities of 100 ppm, prevents the ulcerogenic eVect of copper. Prophylaxis also implies any other procedure that prevents keeping food in the stomach longer, and that reduces the possibility of increasing the acidity of its contents. The addition of antacid compounds that have a certain buVer eVect can be an additional measure toward reducing the risk of this disease. It is necessary to enable the animals’ optimal ambient conditions of accommodation and to carry out the corresponding procedures in all stages of breeding. Possible stress situations (loading, transportation, unloading, introduction into a new herd, and similar) should also be prevented with the application of tranquilizers.

E. Forensic Evaluation Literature that deals with esophagogastric ulcers in swine from diVerent aspects is quite numerous, but there are nevertheless very few data on the elements that determine the duration of this disease. It is known that the course of the disease can be peracute, acute, subacute, and chronic (Curtin et al., 1963; Muggenburg et al., 1964). The peracute course is very brief and the animals die suddenly, in good condition, due to intensive gastrorrhagia. The rapid development of the disease and its brief course are indicated by the fact that piglets aged 6 weeks have died of it (Muggenburg et al., 1967), as well as the observation of clinical signs of the disease and the finding of ulcers in piglets aged only 14 days (Curtin et al., 1963). Exitus sometimes occurs during the acute course of the disease because of progradient ulcer disease, when the process leads to the perforation of the stomach wall and

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the consequently resulting peritonitis (Bussolati and Canese, 1972). The subacute and chronic course can last up to 50 days and end with the death of the swine due to extreme cachexia (Kowalczyk and Muggenburg, 1963). Necrosis can develop very rapidly, in a few minutes only, or much more slowly, in several days. The type of cell as well as the degree of the aggressiveness of the etiological factor are of primary importance in this. Literature data and our own results on the pathomorphological characteristics of esophagogastric ulcers in swine indicate that they can be manifested as acute erosions, subacute ulcers, or chronic ulcers. The time limits of the duration of such changes are not given (Curtin et al., 1963; Fedorov et al., 1977; Muggenburg et al., 1964; Sˇenk and Sˇabec, 1965; Thoonen and Hoorens, 1963). Pathohistological examinations of esophagogastric ulcers undoubtedly indicate the possible evolution of changes from the preulcerous keratinization of the mucosa to the erosive ulcerous processes. The appearance of granulation tissue in the propria and submucosa is taken as a sign of the micromorphological transition of acute to chronic ulcers. In the course of the further duration of the process, the granulation tissue also covers the intermuscular connective tissue of the tunica muscularis, which leads to marked thickenings of the intermuscle septae. Ulcer processes sometimes end with a connective tissue scar, whose formation had certainly been preceded by development over several weeks. Preulcerous erosive changes in the form of smaller surface defects of the mucosa are characterized histologically by dystrophic and necrobiotic changes in surface epithelial cells, with the appearance of neutrophil leukocytes in the propria (Curtin et al., 1963; Thoonen and Hoorens, 1963), which, according to the duration of the process, belongs to the acute course lasting from several hours to several days. In the further course of this still acute condition, larger and deeper erosions develop, when propria edema is developed in addition to the dystrophic‐necrobiotic changes in the epithelium, and macrophages appear along with the infiltration of leukocyte cells (Fedorov et al., 1977). A formed chronic ulcer is characterized, in addition to the progressive penetration of peptic necrosis of the epithelium and propria into the muscularis of the mucosa and submucosa, by changes in the cellular infiltrate, which is located immediately adjacent to the necrotized tissue of the ulcer. Along with the rare neutrophil leukocytes and macrophages, cell elements appear that are otherwise found in young granulation tissue––lymphocytes, plasma cells, and fibroblasts. In the further progress of the chronic course of the disease and the maturing of the granulation tissue, a connective capsule is formed on the ulcer periphery, with dominant fibrocytes and collagen fibers (Fedorov et al., 1977). The forensic evaluation of the changes in the duration of the organization processes is based on the timed inclusion of proliferation and migration of

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parenchymatous cells and fibroblasts, protein synthesis in the extracellular matrix, the creating of new blood vessels (angiogenesis), and the maturing and retraction of the scars. The reparation process begins 24 h after the damage. Fibroblasts and vascular endothelial cells proliferate and create granulation tissue in 3–5 days. The migration of fibroblasts to the site of the damage and their later proliferation are controlled by growth factors (FRPT, EFR, FFR, and TFRb) originating from the macrophages. Some of these growth factors at the same time stimulate the synthesis of collagen and other molecules of the connective tissue. New blood vessels are created through the filling up of the endothelium from the existing blood vessels (angiogenesis) in 3–7 days. The new capillaries have permeable intraendothelial connections, permitting the passage of proteins and erythrocytes into the extravascular space, which is why the granulation tissue is often edematous. Angiogenesis is induced most probably by the basic FFR growth factor, and, according to some authors, by the vascular‐endothelial growth factor (VEFR). Macrophages are always present in the stroma of the granulation tissue, provided there is a corresponding chemoattractant stimulation and there are neutrophils, eosinophils, and leukocytes, within a period of 3–7 days. As of this period, the number of blood vessels is reduced, and the number of fibroblasts, the collagen density, and the amount of extracellular matrix are increased. The appearance of leukocytes can be established after several minutes; they are most numerous at up to 7 days as well as during chronic processes, which last for months. Macrophages and fibroblasts appear after the third day, and during the process at up to 7 days at least, and longer, and elastic fibers are formed only after the fourth week. The finding of lymphocytes indicates that the process has lasted at least 7 days, and of plasmocytes, 10 days. The extremely long duration of the organization process of 3 or more months is established with the finding of collagen fibers that refract light twice. Swine deaths due to esophagogastric ulcers contribute to economic damage on a farm or some other swine breeding facility, and they also have forensic significance in certain cases of sales. Due to the absolutely disguised course of the disease and the possibility of a sudden lethal outcome, this disease meets two of the three basic criteria for evaluation as a material fault in the animal, in keeping with national legal regulations (Aleksic´ et al., 1984). Thus, in addition to the covertness and significance of the disease, this third element of the evaluation of its duration––the existence of stomach ulcers in swine before sales, or the development of pathological changes only after an animal has changed owners––can be determined only on the grounds of the changes found during autopsy. Pathomorphological characteristics of spontaneously developed ulcers in swine provide the possibility that its duration can be determined in chronic courses of the disease within limits of at least

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6 weeks and up to 2 or at most 3 months. These are the size and depth of the defects on the mucosa of the esophagogastric region, rounded and raised edges of the ulcer and a base with a granulated appearance, a pathohistological finding of a reactive inflammatory process in the neighborhood of the ulcer, changes in blood vessels, and the proliferation of groups of fatty cells in granulation or already mature connective tissue. With the development of erosive changes in a hyperkeratotically altered mucosa, the evaluation of the duration can range between 14 and 21 days.

IV. Concluding Remarks Spontaneous ulcers, usually of the stomach, commonly occur in many domestic animals. Some of these lesions are chronic and they may occur in either the glandular or squamous‐lined regions of the stomach. As with human disease, the pathogenesis in domestic animals is multifactorial, poorly understood, and variable between and within species. Environmental stress and dietary factors are extremely important in ulcer disease in swine. It has been shown that the Helicobacter spp. is strongly associated with naturally occurring ulcer and preulcer lesions of the pars esophagea in swine, which raises the possibility that Helicobacter spp. is an important factor in the pathogenesis of these lesions. The dynamics of the development of esophagogastric ulcers imply hyperplastic lesions (parakeratosis and hyperkeratosis), keratolysis, erosions, peptic necrosis, and the development of ulcers with all the characteristics of peptic ulcerations in other localities. In addition, K6 is expressed in association with the mucosal changes. The pattern of intermediate filaments of keratin suggests that epithelial proliferation, which leads to visible hyperkeratosis, is at the essence of gastric ulcers in swine. References Aleksic´, Z. (1987). Morfolosˇka i histohemijska ispitivanja zˇlezdane sluznice zˇeluce svinja sa preulceroznim i ulceroznim lezijama ezofagealnog podrucˇja Dissertation, Beograd. Aleksic´, Z., and Dukic´, B. (1984). Odgovornost za naknadu sˇteta prouzrokovanih opasnim stvarima i opasnom delatnosˇc´u po Zakonu o obligacionim odnosima u oblasti veterinarske delatnosti. Vet. gl. 38(2), 121–127. Aleksic´, Z., and Knezˇevic´, M. (1989a). Histohemijska analiza zˇeludacˇnih mucina kod ezofagogastricˇnog ulkusa u svinja. Zb. XII Jugoslovenskog savetovanja vet. 91. Aleksic´, Z., and Knezˇevic´, M. (1989b). Ispitivanje odnosa kiselih i neutralnih mucina u sluznici zˇeluca svinja sa eksperimentalno izazvanim ezofagogastricˇnim ulkusom. Zbornik radova VI savetovanja veterinara Srbije, Zlatibor, 130–134.

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Mastronardi, M. A. (1964). Propisitio delazione ulcerogena della reserpina sul tubo gastro‐ enteritico. Acta Med. Vet. Napoli 10, 441–449. ˇ ., and Milic´, D., Stokic´, Z., Levajic´, D., Milinovic´, M., Grus, I., Loncˇarevic´, A., Stankovic´, C Pavlovic´, A. (1968). Problem ezofagogastricˇnog ulkusa kod svinja na farmama otovorenog tipa. Acta Galen. 8, 7–9. Muggenburg, B. A., Reese, N., Kowalczyk, T., Grummer, R. H., and Hoextra, W. G. (1964). Survey of the prevalence of gastric ulcers in swine. J. Am. Vet. Res. 25, 1673–1678. Muggenburg, B. A., Kowalczyk, T., Hoextra, W. G., and Grummer, R. H. (1966a). Experimental production of gastric ulcers in swine by reserpine. Am. J. Vet. Res. 27, 1663–1669. Muggenburg, B. A., Kowalczyk, T., Reese, N., Hoextra, W. G., and Grummer, R. H. (1966b). Experimental production of gastric ulcers in swine by histamine in mineral oil‐beeswax. Am. J. Vet. Res. 27, 292–299. Muggenburg, B. A., Reimann, E. M., Kowalczyk, T., and Hoextra, W. G. (1967). EVect of reserpine and histamine in mineral oil beeswax vehicle on gastric secretion in swine. Am. J. Vet. Res. 28, 1427–1435. Muggenburg, B. A., Kowalczyk, T., and Olson, W. (1971). EVect of ambient temperature on gastric lesions and gastric secretion in swine. Am. J. Vet. Res. 32, 603–608. Nappert, G., Vrins, A., Beauregard, M., Vermette, L., and Lariviere, N. (1990). Radioimmunoassay of serum pepsinogen in relation to gastric (pars oesophagea) ulceration in swine herds. Can. J. Vet. Res. 3, 390–393. Nelson, W. (1966). Nitrite toxicosis and the gastric ulcer complex in swine. Part I. Nitrite toxicosis. Part II. Gastric ulcers complex. Dis Abstr. Int. 26, 40–41. Nuner, A. J., Perry, T. W., Pickett, R. A., and Cuetin, T. M. (1966). Expanded or heat‐ processed fractions of corn and their relative ability to elicit esophagogastric ulcers in swine. J. Anim. Sci. 26, 518–525. Olivier, L., and Houix, Y. (1969). Incidence de l’ulcere gastrooesophagien dans un tropeau experimental porcin et ses repercussions sur la croiasance et la qualite des caracasses. Ann. Zootech. 18, 209–219. Otto, K., and Hugo, S. (1960). In ‘‘Lehrbuch der histologie und vergeleichenden Anatomie der Haustiere’’ (A. Trautmann and J. Fiebiger, Eds.), pp. 234–244. Springer‐Verlag, Berlin. Palavicin, G., Aureli, G., and Castellani, A. (1971). Chemical changes in the gastric mucin of the pig with spontaneous or experimental gastric ulcer. Atti. Soc. ital. aci. vet. 24, 209–212. Panasjuk, B. B., Skiljarov, J. P., and Karpenko, L. N. (1979). Ultrastrukturnie i mikrohemicˇeskie procesi v zˇeludocˇnih zˇeleza, 94–101. Pearse, A. G. E. (1960). Comon cytochemical properties of cells producing polypeptide hormones, with particular reference to calcitonin and the thyroid cells. Vet. Res. 79, 587–590. Pearse, A. G. E., Julia, M., Polak, J. M., Bloom, S. R., Adams, C., Dryburgh, J. R., and Brown, J. C. (1974). EnterochromaYn cells of the mammalian small intestine as the source of motilin. Virchows Arch. B Cell Pathol. 16, 111–120. Pearse, A. G. E., Polak, J. M., and Bloom, S. (1977). The newer gut hormones: Cellular sources, physiology, pathology, and clinical aspects. Gastroenterology 72, 746–761. Penny, R. H. C., Edwards, M. J., and Mulley, R. (1972). Gastric ulcer in the pig, a new South Wales abattoir survey of the incidence of lesions of the pars oesophagea. Br. Vet. J. 128, 43–49. Perry, T. W., Jimenez, A. A., Shivrly, J. E., Piccett, R. A., Curtin, T. M., and Beeson, W. B. (1962). EVect of type of ration on the incidence of swine gastric ulcers. J. Anim. Sci. 21, 1008–1014. Petrosjan, F. R. (1975). Materiali VI Vsesojuznoj konferencii po patologicˇeskoj anatomii zˇivotnih (zb. radova), 223–225, Talin.

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Molecular Mechanism of Phase I and Phase II Drug‐Metabolizing Enzymes: Implications for Detoxification Takashi Iyanagi Biometal Science Laboratory, RIKEN SPring‐8 Center, Harima Institute, Hyogo 679‐5148, Japan

Enzymes that catalyze the biotransformation of drugs and xenobiotics are generally referred to as drug‐metabolizing enzymes (DMEs). DMEs can be classified into two main groups: oxidative or conjugative. The NADPH‐cytochrome P450 reductase (P450R)/cytochrome P450 (P450) electron transfer systems are oxidative enzymes that mediate phase I reactions, whereas the UDP‐glucuronosyltransferases (UGTs) are conjugative enzymes that mediate phase II enzymes. Both enzyme systems are localized to the endoplasmic reticulum (ER) where a number of drugs are sequentially metabolized. DMEs, including P450s and UGTs, generally have a highly plastic active site that can accommodate a wide variety of substrates. The P450 and UGT genes constitute a supergene family, in which UGT proteins are encoded by distinct genes and a complex gene. Both the P450 and UGT genes have evolved to diversify their functions. This chapter reviews advances in understanding the structure and function of the P450R/P450 and UGT enzyme systems. In particular, the coordinate biotransformation of xenobiotics by phase I and II enzymes in the ER membrane is examined. KEY WORDS: Drug‐metabolizing enzymes, Cytochrome P450 reductase, Cytochrome P450, Microsomal electron transfer system, Endoplasmic reticulum, UDP‐ glucuronosyltransferases, Supergene family, UGT1 gene complex, Antley‐Bixler syndrome, Crigler‐Najjar syndrome. ß 2007 Elsevier Inc.

I. Introduction Almost all drugs that undergo metabolic transformation are converted to metabolite, which are more polar than the parent compound. Biotransformation not only promotes drug elimination but also often results in inactivation International Review of Cytology, Vol. 260 Copyright 2007, Elsevier Inc. All rights reserved.

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0074-7696/07 $35.00 DOI: 10.1016/S0074-7696(06)60002-8

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of pharmacological activity, thereby changing the overall biological properties of the drug (Wilkinson, 2001). However, a number of relatively inert xenobiotics, which are foreign to living organisms (Greek; xenos and biot, for ‘‘stranger to life’’), has been found to be converted by enzymes in the body to extremely toxic products. DMEs, which can be involved in complex metabolic networks of the body, are classed as phase I or phase II enzymes. Phase I enzymes often catalyze oxidation, reduction, and hydrolysis reactions. Most phase II enzymes catalyze conjugation reactions: UDP‐glucuronosyltransferases (UGTs), sulfotransferases (SULTs), or glutathione S‐transferases (GSTs). Drugs are often metabolized by sequential reactions involving phase I and II enzymes. The time taken for a drug to be cleared from the body is a function of both the rate of biotransformation and excretion. The major role of P450s is to introduce polar functional groups into nonpolar molecules. Conjugating enzymes catalyze the addition of more polar functional groups to the drug, such as glucuronate, sulfate, glutathione, or amino acids. NAD(P)H: quinone:oxidoreductase (also called DT‐diaphorase), methyltransferase, and acetyltransferase are also classed as phase II enzymes. Sequential biotransformations by both the P450R/P450 system and UGTs constitute one of the major routes for drug metabolism. These sequential reactions might be facilitated by the close spatial association of the enzymes on the endoplasmic reticulum (ER). The metabolites generated by phase I and II reactions are excreted from the body with the aid of membrane eZux pumps that include the multidrug resistance‐associated proteins (phase III reactions). The P450R/P450 system and UGTs play a vital role in the metabolism and detoxification of xenobiotic (exogenous) and endobiotic (endogenous) compounds. The P450 and UGT superfamily of genes encode proteins that metabolize a diverse set of substrates. P450 proteins are encoded by distinct genes, whereas the P450R protein is encoded by a single gene. Thus, P450R can donate electrons to all microsomal P450s. In contrast, UGT proteins are encoded by both distinct genes and a complex gene. Both the P450 and UGT genes have evolved to diversify their functions (Gibbs et al., 2004). The combinatory pharmacogenetics of these enzymes is an increasingly important research field in clinical medicine (Wilke et al., 2005).

II. Phase I: NADPH‐Cytochrome P450 Reductase (P450R)/Cytochrome P450 (P450) System Phase I enzymes (functionalization reactions), which mediate oxidation, reduction, or hydrolysis reactions, introduce a functional group (‐OH, ‐SH, ‐NH2, or ‐COOH) into the drug molecule. The P450R/P450 is a major oxidative enzyme system (Gibson and Skett, 2001). The P450‐containing microsomal electron

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transfer system catalyzes the oxidation of drugs and xenobiotics. Although there are numerous functional P450 genes in mammals (e.g., 84 in rat, 87 in mouse, 57 in human) (Gibbs et al., 2004), there is only one P450R gene in each species. P450 genes are distributed on several chromosomes, although they are often found in clusters. The human genome project has identified 57 functional P450 genes: seven encode mitochondrial enzymes, all of which play key roles in sterol biosynthesis, and 50 encode microsomal enzymes (Guengerich, 2005; Nelson et al., 2004). Of the 50 microsomal enzymes, 20 participate in the biosynthesis of endobiotic substrates, such as steroids and eicosanoids; 15 principally metabolize xenobiotic compounds; and 15 are orphan enzymes (named because their substrates have not been identified). P450R can donate electrons to 50 microsomal P450s, which are located in the ER. In this section, the structure/function of the microsomal electron transfer system is described. In addition, the diVerences between P450R and nitric oxide synthase (NOS) reductase domains are discussed.

A. Historical Perspectives In the early 1950s, little was known about the oxidative enzymes involved in metabolizing drugs and xenobiotics. Mason et al. (1955), Hayaishi et al. (1955), and Hayano et al. (1955) independently demonstrated direct substrate incorporation of molecular oxygen. These pioneering experiments opened a new field in the area of biological oxidation, including cytochrome P450s. Molecular oxygen is metabolized by three broad classes of enzymes: (1) dioxygen transferases, (2) mixed‐function oxidases, and (3) electron‐ transfer oxidases (Mason, 1957). The microsomal deamination of amphetamine (Axelrod, 1955) and dealkylation of aminopyrine (Gillete et al., 1957; La Du et al., 1955) requires the reduced form of nicotinamide adenine dinucleotide phosphate (NADPH) and molecular oxygen (O2). Enzymes of the liver microsomes are of major importance in the detoxification of many drugs and foreign organic compounds. In the 1950s–1960s, these enzyme systems were shown to perform a variety of reactions such as the hydroxylation of aromatic compounds, side chain oxidation of barbiturates, and deamination of amines. These reactions were characterized as a mixed‐ function oxidation, in which the enzyme system catalyzes the consumption of one molecule of oxygen/molecule of substrate (RH); one atom of this oxygen molecule inserts into the product (ROH), and the other undergoes two equivalents of reduction (Eq. 1). NADPH þ RH þ O2 þ Hþ ! NADPþ þ ROH þ H2 O

ð1Þ

Klingenberg (1958) and Garfinkel (1958) discovered a novel carbon monoxide‐binding pigment with an optical absorption peak at 450 nm in

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liver microsomes. Omura and Sato (1962, 1964a,b) purified this pigment as a P420 form from liver microsomes and showed that it was a cytochrome, which they named cytochrome P450 (Kresge et al., 2006; Omura, 2005). Hashimoto et al. (1962) demonstrated the electron spin resonance detectable ‘‘microsomal Fex signal’’ at g ¼ 2.25 in liver microsomes, derived from a low‐spin ferric hemoprotein, which was preferentially reduced by NADPH. Mason et al. (1965) suggested that a more active enzyme toward P450 and microsomal Fex reduction is TPNH (NADPH)‐cytochrome c reductase, which was first identified by Horecker (1950) as an NADPH‐specific cytochrome c reductase, and characterized by Williams and Kamin (1962) and Phillips and Langdon (1962). Using submicrosomal particles containing P450, Miyake et al. (1968) demonstrated that the microsomal Fex signal is derived from low‐spin ferric P450. Estabrook et al. (1963) showed that this pigment from the photoactivation spectra of CO‐inhibited mixed‐function oxidations appears to be the functional site of several microsomal mixed‐function oxidases. Lu and Coon (1968) demonstrated that microsomal fatty acid hydroxylase requires three fractions containing P450, cytochrome c reductase activity, and phospholipids for activity. Iyanagi and Mason (1973) found an air‐stable g ¼ 2 signal in liver microsomes, which was increased by the addition of NADPH. This signal was derived from air‐stable semiquinone of the NADPH‐cytochrome c reductase. Furthermore, the enzyme was shown to contain one molecule of FAD and FMN per protein molecule, with each flavin performing an individual function. The spin concentrations of air‐stable semiquinone and their spectra were compared with those of flavodoxin (Iyanagi et al., 1974). The data indicated that the enzyme contained a flavodoxin‐type flavin, which is a FMN‐containing small bacterial flavoprotein. Flavodoxin can substitute for the low‐potential ferredoxin during growth under low‐iron conditions (Knight and Hardy, 1966; Mayhew et al., 1969). An iron sulfur protein with g ¼ 1.94 signal could not be detected in liver microsomes (Miyake et al., 1967). These observations strongly suggested that NADPH‐cytochrome c reductase participates as an electron carrier in microsomal electron transfer. Iyanagi et al. (1974) postulated that this enzyme could directly reduce cytochrome P450, which was named NADPH‐cytochrome P450 reductase (P450R). These studies led to the discovery of a new microsomal electron transfer system, including P450R and P450 (Fig. 1). B. P450R/P450 Electron Transfer System 1. Electron Transfer System The mixed‐function oxidase system of liver microsomes was resolved into three fractions, consisting of P450R, P450, and a lipid component (Lu and Coon, 1968; Lu et al., 1969). P450R can directly reduce P450s in a

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FIG. 1 The electron transfer systems in the mixed‐function oxidases. (A) flavodoxin; (B) ferredoxin reductase; (C) ferredoxin; (D) NADPH‐cytochrome P450 reductase (P450R); (E) NADH‐cytochrome b5 reductase (b5R); (F) cytochrome b5 (b5); (G) nitric oxide synthase (NOS) (dimmer structure); H4B, tetrahydrobiopterin.

purified reconstituted system (Imai et al., 1977; Iyanagi et al., 1978; Strobel and Dignam, 1978; Vermilion and Coon, 1974; Yasukochi and Masters, 1976). Taniguchi et al. (1979) reported a reconstituted system in phosphatidylcholine vesicles. These studies confirmed that the microsomal electron transfer system consists of two components: P450R and P450. The low potential flavin, FAD, accepts two reducing equivalents from NADPH and the high potential flavin, FMN, acts as a one‐electron carrier for the net two‐ electron transfer from NADPH to P450 (Iyanagi et al., 1981; Vermilion et al., 1981). The cDNA cloning (Porter and Kasper, 1985; Yamano et al., 1989), direct complete amino acid analysis (Haniu et al., 1986, 1989) and crystallographic structure of P450R (Wang et al., 1997) confirmed that the protein evolved by fusion of two ancestral genes encoding proteins related to ferredoxin‐NADPþ reductase (FNR) and flavodoxin. Bredt et al. (1991) isolated the cDNA of neuronal nitric oxide synthase (nNOS), which is localized to neurons throughout the peripheral and central nervous system (CNS). The C‐terminal reductase domain of nNOS bears 58% sequence similarity with P450R. In the case of the microsomal desaturase system, the cytochrome b5 (b5) can function as a one‐electron carrier. In contrast, the mitochondrial system comprises adrenodoxin reductase (a single subunit, mono–FAD‐containing enzyme) and adrenodoxin (adrenal ferredoxin; an iron ferredoxin‐type redox protein), which together function as an electron carrier from NADPH to P450 (Kimura

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and Suzuki, 1967; Omura et al., 1966). In general, the bacterial systems consist of three components, including a ferredoxin. This fact suggests that the mitochondrial P450 electron transfer system in eukaryotes is derived from bacteria. However, Bacillus megaterium cytochrome P450BM3 (P450BM3) is a single component fatty acid hydroxylase. It is composed of an N‐terminal P450 mixed‐function oxygenase domain fused to an FMN‐ and FAD‐binding reductase domain, which is related to mammalian P450R (Narhi and Fulco, 1987). These electron transfer events indicate that a one‐electron carrier is necessary for the sequential electron transfer from a two‐electron donor (NAD[P]H) to a P450, which is a one‐electron acceptor (Fig. 1). In principle, the sequence of electron transfer for mixed‐function oxidases is summarized as follows: two‐electron donor ! dehydrogenase flavin ! one‐electron carrier ! oxygenase (P450) (Fig. 1). In these electron transfer systems, the FMN domains of P450R and NOS can also function as a one‐ electron carrier. These electron transfer systems require three functions: (1) dehydrogenase from NAD(P)H, (2) one‐electron carrier, and (3) stepwise activation of molecular oxygen by an oxygenase. A ‘‘step down’’ reaction from a two‐electron donor to a one‐electron acceptor is an essential step in biological oxidations. The oxygenases accept electrons from a constant oxidation‐reduction potential. 2. Structure of P450R and nNOS Reductase Domain NADPH‐cytochrome P450 reductase (P450R) is a 78 kDa (678 aa for rat enzyme) flavoprotein associated with the cytoplasmic surface of the ER and the outer membrane of the nuclear envelope in eukaryotic cells (Gonzalez and Kasper, 1981). The gene expression of functional domains (Smith et al., 1994) and the crystal structure of rat P450R (Wang et al., 1997) clearly indicate that the enzyme is composed of four domains: an FMN‐binding domain (residues 70–225), the connecting domain (residues 325–450) and the FAD‐ and NADPH‐binding domains (Fig. 2). The connecting domain is inserted in the NADPH/FAD domain. The enzyme also contains a membrane‐binding domain at the N‐terminus (Fig. 2). The structure of the FMN‐binding domain is similar to that of flavodoxin, whereas the two C‐terminal dinucleotide‐binding domains are structurally homologous to those of ferredoxin‐NADPþ reductase (FNR), NADPH‐flavodoxin reductase and NADH‐cytochrome b5 reductase (b5R) (Porter and Kasper, 1985; Wang et al., 1997). The distance between the isoalloxazine components of ˚ , indicating direct electron transfer between the dimethylthe flavins is 4 A benzene edges of the two flavin molecules. A high degree disorder in the FMN domain, observed in the crystal structure of P450R, suggests that this domain retains a considerable degree of mobility. Mutant studies have been performed to investigate the nature of the intramolecular interactions during

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A

B

CD

CD

CT

βF AI

FAD/NADPH domain

FAD/NADPH domain

FMN domain

C

FMN domain

FAD/NADPH domain 1 P450R M

678 FMN CD

1 nNOS PDZ

FAD/NADPH

Heme(Fe)

FMN CaM

AI

NBD

1434

FAD/NADPH CT

FIG. 2 The domain structure of NADPH‐cytochrome P450 reductase (P450R) (A), neuronal nitric oxide synthase (nNOS) reductase domain (B), and functional domains of P450R and nNOS (C). M, Membrane‐binding domain; PDZ, PDZ domain; CaM, CaM‐binding region; AI, autoinhibitory domain; CD, connecting domain; CT, C‐terminal motif; bF, b finger; NBD, highly conserved nucleotide‐binding domain in the P450R family (Wang et al., 1997). A and B are cited from Protein Data Bank Codes 1AMO and 1TLL, respectively.

catalysis. Superimposition of the mutant and wild‐type structures revealed ˚ to 5.8 A ˚ (Hubbard et al., 2001), the flavin–flavin distance varies from 3.9 A strongly suggesting movement of the FMN domain during catalysis. Nitric oxide (NO) has diverse biological functions and is generated in mammals by NOS enzymes. Three NOS isozymes participate in distinct physiological processes (Roman et al., 2002). Inducible NOS (iNOS) is involved in the immune system when NO is produced as a cytosolic agent. Endothelial NOS (eNOS) is involved in the maintenance of blood pressure, whereas nNOS participates in neuronal transmission. All NOSs are homodimeric enzymes that catalyze an NADPH‐ and O2‐dependent oxidation of L‐arginine (L‐Arg) to L‐citrulline (L‐Cit) and NO (Fig. 1). Each NOS consists of a C‐terminal reductase domain that contains binding sites for FAD, FMN, and NADPH, an intervening calmodulin‐binding domain, and an N‐terminal P450‐like domain that contains binding sites for iron protoporphyrin IX (heme), 6R‐tetrahydrobiopterin (H4B),

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TAKASHI IYANAGI

and Arg. The structure of rat nNOS reductase domain, which lacks the calmodulin (CaM)‐binding domain, has been reported by Garcin et al. (2004) and is very similar to that of rat P450R (Wang et al., 1997). The crystal structure of rat P450R and rat nNOS reductase domains is considered representative of this family of proteins (Fig. 2). Although the overall structural organization of P450R and nNOS reductase domain is similar, significant diVerences are evident in nNOS. Interestingly, the autoinhibitory (AI) motif is inserted within the FMN domain of rat nNOS (residues 831–870) and bovine eNOS (residues 600–640) reductase domains (Salerno et al., 1997), and is located between the FMN‐ and NADPH‐binding sites (Garcin et al., 2004). Furthermore, the b‐finger (residues 1070–1080) and N‐terminal b‐loop‐helix (residues 963–986) are found on the rat nNOS structure (Zhang et al., 2001). The distance between the FAD and FMN ˚ , and the position of the two flavin cofactors diVer moieties is less than 5 A significantly from that of P450R (Fig. 3). The air‐stable (neutral) semiquinone form is characteristic of both the P450R and NOS reductase domains and contain the oxidized flavin (FAD) and semiquinone form of FMN (FMNH ) in equimolar amounts. In the flavodoxin, the FMN semiquinone form is stabilized by the interaction with apoprotein. In the P450R and NOSs, the value of the semiquinone formation constant Ks is larger than unity, indicating an increase in the separation between the oxidized/semiquinone couple (Em.1) and semiquinone/fully reduced couple (Em.2) in each flavin (Iyanagi, 2005a,b). This stabilization of neutral semiquinone is due to hydrogen bond formation between the polypeptide backbone of the protein and the N(5) of the reduced FMN, lowering its activity. Specifically, FMN hydrogen bonds to Gly141 in rat P450R, and Gly810 in rat nNOS, whereas FAD hydrogen bonds to Ser457 in rat P450R and Ser1176 in rat nNOS (Garcin et al., 2004; Wang et al., 1997). However, the fully reduced form is destabilized by constraints from the unfavorable planar conformation, and its activity is increased. Therefore, this state has more activity than that of the semiquinone. By contrast, the semiquinone of the FMN domain of bacteria P450BM3, in which a hydrogen bond at the (N)5 is formed to the peptide nitrogen of Asn537, stabilizes the anionic red semiquinone (FMN ) (Hanley et al., 2004). Because of the stabilization of anionic semiquinone, this enzyme may have a high turnover rate. The anionic red semiquinone form is also observed in the b5R (Iyanagi, 1977; Iyanagi et al., 1984; Kobayashi et al., 1988; Marohnic et al., 2003), but its neutral blue semiquinone form is partially stabilized in the mutant of T66V (Kimura et al., 2003), which is positioned near the (N)5 atom of the isoalloxazine ring of FAD. In this mutant, b5R activity is decreased. The reduction potentials of the individual one‐electron redox couples (Em.1 and Em.2) of FAD and FMN of P450R have been reported (Iyanagi et al., 1974; Munro et al., 2001). In both FAD and FMN, the semiquinone formation

_

_

43

PHASES I AND II DRUG‐METABOLIZING ENZYMES

A

B R1400

W677 Y178

R454

F1395

R1173

Y889

Y1175

Y456 Y455 FAD

F809

Y1174

Y140 FMN

FAD

FMN

FIG. 3 The structures of the FAD‐ and FMN‐binding sites of P450R (A) and nNOS reductase domain (B). In B, arrows indicate the shift and rotation of the plane of FMN molecule from that of P450R. A and B are cited from Protein Data Bank Codes 1AMO and 1TLL, respectively.

constant is larger than unity. In the case of NOSs (Gao et al., 2004; Ghosh et al., 2006; Noble et al., 1999), the overall redox potentials are very similar, although the values for the FAD domains are greater than those of P450R. In both enzymes, the air‐stable semiquinone form, FAD–FMNH has a relatively high reduction potential and low reactivity with electron acceptors. Therefore, the semiquinone/fully reduced couple (FMNH /FMNH2), could function as a one‐ electron carrier in the catalytic cycle for both the FAD–FMN pairs in P450R and NOSs. The couples (FMNH /FMNH2) of each enzyme are 270 mV for P450R (Iyanagi et al., 1974), 180 mV for iNOS, 180 mV for nNOS, and 210 mV for eNOS (Ghosh et al., 2006). The first and second electrons from the reductase to P450 or P450‐like hemoprotein are sequentially transferred from these states, which can donate an electron at a constant oxidation‐reduction potential. However, in the bacterial P450BM3 the oxidized/semiquinone couple (FMN/FMN ) functions as a one‐electron carrier in the catalytic cycle (Murataliev et al., 2004; Sevrioukova et al., 1999), in which the anionic red semiquinone form can donate electrons to P450. The couples, FMN/FMN and FMN /FMNH2 are 240 mV and 160 mV, respectively (Hanley et al., 2004). The redox potential is unique among flavodoxin‐like domains, as compared with those of P450R and NOSs. The oxidation‐reduction potentials of the flavin cofactor in flavoproteins are controlled by a variety of noncovalent flavin–protein interactions (Mayhew and Ludwig, 1975; Swenson and Krey, 1994).

_

_

_

_

_

_

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TAKASHI IYANAGI

3. Evolutionary Aspects Mammalian P450‐containing electron transfer systems are divided into two types: mitochondrial and microsomal (Fig. 1). The mitochondria of animal species arose via the incorporation of purple bacteria into eukaryotic cells, whereas the ER could have arisen from other eubacterial species, possibly of the Gram‐positive type. The microsomal and mitochondrial P450s separated about 950 million years ago, which is close to the accepted time of divergence between the plant and animal kingdoms at about 1000 million years ago (Lewis, 2001; Lewis et al., 1998). This is also coincident with the development of sexual reproduction. The mitochondrial P450s are crucial for the biosynthesis of steroid hormones, whereas microsomal P450s are crucial for the metabolism of xenobiotics, such as plant toxins, prostanoids, and eicosanoids. Indeed, this is a natural consequence of more complex multicellular organisms such as plants, fungi, and primitive animals (Lewis, 2001). The mitochondrial and microsomal P450s have also evolved synergistically for the biosynthesis of endobiotics, such as steroid hormones and vitamin D. The domain families have been extensively duplicated within a genome and combined with diVerent domain partners giving rise to diVerent multidomain proteins (Orengo and Thornton, 2005). It is possible to speculate about the evolutionary development of microsomal P450 redox systems and NOSs in terms of the structure and function of the one‐ electron carrier, ferredoxin, and flavodoxin (Fig. 4). The structure and function of the FAD‐ and FMN‐binding domains of P450R and NOS isozymes show a striking evolutionary relationship with plant FNR and bacterial flavodoxins in terms of electron transfer and its regulation. It is thought that the ancestor of these enzymes might have evolved from at least four discrete genes, encoding ferredoxin or flavodoxin reductase (FAD), ferredoxin (2Fe2S), flavodoxin (FMN), and a heme (Fe) domain (Fig. 4). Bacterial flavodoxin (FMN) can substitute for the low‐potential ferredoxin (2Fe2S) during growth under low‐iron conditions. The flavodoxin reductase, a FAD containing bacterial flavoprotein, catalyzes the reversible transfer of electrons between NADPH and flavodoxins or ferredoxins (Ingelman et al., 1997). Flavodoxin reductase and flavodoxin are involved in cobalamin‐dependent methionine synthesis (Hall et al., 2001). However, in the mammalian system, the methionine synthase reductase has a similar prosthetic group with that of P450R (Olteanu and Banerjee, 2001; Olteanu et al., 2004; Wolthers et al., 2003), but it is a soluble protein. The other proteins, including the a‐subunit of sulfite reductase (Sulfite R) and P450BM3 carry domains homologous to flavodoxin and flavodoxin reductase or FNR on a single polypeptide chain. It has been hypothesized that these enzymes arose from a gene fusion of flavodoxin and flavodoxin reductase or FNR. The structure of flavodoxin, in which the dimethylbenzene ring of FMN molecule is exposed to solvent, is also superimposable on those of the

PHASES I AND II DRUG‐METABOLIZING ENZYMES

45

FIG. 4 A model for the evolution of functional domains in P450R, P450s, and nitric oxide synthase genes. A–D indicate ancestral domains of each gene: A, heme domain; B, FMN domain; C, FAD domain; D, Fe‐sulfur cluster domain. Fed, ferredoxin; Fed R, ferredoxin reductase; Sulfite R, sulfite reductase; P450BM3, Bacillus megaterium P450BM3. The number of functional isozymes is shown in parentheses.

a‐subunit of Sulfite R, P450R, and NOS FMN‐binding domains (Garcin et al., 2004; Sibille et al., 2005; Wang et al., 1997). The NADPH/FAD domain for both enzymes is also superimposable on that of FNR (Jachymova et al., 2005; Mayoral et al., 2005). In the modeling of the FNR–flavodoxin complex, P450R is a good example of an eYcient interflavin electron transfer between FAD and FMN ˚ (Figs. 2, 3), the shortest distance between the two flavin rings being 4.1 A (Mayoral et al., 2005). No intervening residues are present between the two cofactors, thereby allowing direct electron transfer. In the complexes of FNR–ferredoxin, the distance between the [2Fe‐2S] cluster of ferredoxin ˚ (Kurisu et al., 2001). In the and the dimethylbenzene edge of FAD is 6.0 A complexes of adrenodoxin reductase‐adrenodoxin, in which an electron is transferred from the pyrimidine ring of FAD to the iron center, the distance between the [2Fe‐2S] cluster of adrenodoxin and the isoalloxazine ring of ˚ , in which two possible electron transfer tunneling pathways FAD is 10 A have been proposed on the basis of the crystal structure (Muller et al., 2001). Taken together, the data suggest that the distance between FAD and FMN is less than that between the FAD and [2Fe‐2S] cluster in these redox systems.

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TAKASHI IYANAGI

In addition, P450R acquired the membrane‐binding domain for eYcient electron transfer with P450 on the ER membrane. NOS comprises a single soluble enzyme, in which the reductase FAD–FMN domain and oxygenase heme‐domain are fused, together with a regulatory motif (Figs. 2, 4). The P450R and NOS reductase proteins are presumably derived from an ancestral FAD‐ and FMN‐containing flavoprotein (Ghosh and Salerno, 2003). The FAD can function as a dehydrogenase, whereas FMN is a one‐ electron carrier (Fig. 1). Although the partner to the FAD domain is a flavodoxin, alternative combinations of one‐electron carrier are also possible (e.g., ferredoxins and cytochromes). The functional significance of P450R and NOS having a flavodoxin domain is unclear, although it could be related to the degree of interaction between the various redox centers. Interaction between the edges of the dimethylbenzene rings of the two flavin molecules may be favored because it is less hindered than an equivalent interaction between a flavin and a [2Fe‐2S] cluster, the latter being buried within the protein by amino acid residues acting as ligands. However, a novel flavohemoprotein, which contains a cytochrome b5‐like domain at the N‐terminus and a b5R‐like domain at the C‐terminus, has been identified in the ER membrane, although its function remains unknown (Zhu et al., 2004). The rat P450R gene comprises 16 exons; exons 2 and 3 encode the membrane anchor region, exons 4–7 the FMN‐binding domain, and exons 8–16 the FAD/ NADPH‐binding domain (Porter et al., 1990). Comparative analysis of the intron splice location between rat P450R and the human NOS genes indicates that the three human NOS genes are derived from a common ancestral gene by duplication. Moreover, the analysis also showed that the NADPH/FAD‐ and FMN‐binding domains of the P450 and NOS systems display similarity (Hall et al., 1994). Consequently, evolutionary transformation of the cofactor binding sites can occur without major structural changes. nNOS have acquired additional regulatory sequences that control enzyme activity: CaM‐binding, AI, b‐finger, and C‐terminal motifs (Roman et al., 2000). The iNOS isozyme does not contain the AI motif and has a shorter C‐terminal tail than that of the nNOS and eNOS isozymes. However, the oxygenase domains of NOSs do not reveal any sequence homology with known P450s, although they have a common cysteine residue as the proximal thiolate ligand (Masters, 2005; Omura, 2005). This suggests that the origin of the NOS oxygenase domain may be diVerent from those of microsomal or mitochondrial P450s. Proteins homologous to the mammalian NOS oxygenase domain have been found in prokaryotes. One example from Bacillus subtilis has been demonstrated to produce nitric oxide when incubated with NADPH and a mammalian NOS reductase domain (Adak et al., 2002). This suggets that the bacterial electron transfer system may comprise the flavodoxin‐type reductase (FAD) and flavodoxin (FMN). It is hypothesized that the mammalian NOSs are fusion proteins of

47

PHASES I AND II DRUG‐METABOLIZING ENZYMES

the bacterial oxygenase domain and reductase domain from sulfite reductase flavoprotein (Zemojtel et al., 2003). Although the complex multidomain structure of diVerent higher eukaryotic NOSs is the result of several gene fusions, the structure of both P450R and NOSs has evolved synergistically. 4. Mechanism a. Catalytic Cycle of P450R P450R catalyzes the transfer of electrons from NADPH to P450. In this system, the electron transfer is divided into three steps: (1) direct hydride transfer from NADPH to FAD, (2) interflavin electron transfer from FAD to FMN, and (3) electron transfer to electron acceptors, including P450s. In NOSs, these steps may be activated by CaM‐binding. The reduction process begins with the formation of NADPþ‐FADH2‐FMN via hydride transfer from enzyme‐bound NADPH, followed by an interflavin one‐ electron transfer from FADH2 to FMN yielding a disemiquinone species (FADH ‐FMNH ). Oxidized FAD then accepts electrons from a second molecule of NADPH during the subsequent interflavin electron transfer, resulting in a four electron‐reduced form (NADPþ‐FADH2‐FMN2). These half‐reactions have been studied in detail (Gutierrez et al., 2001, 2002; Iyanagi et al., 1981). In this case, the steps are in equilibrium distribution, the redox state being determined by the relative redox potentials (Backes et al., 1998; Iyanagi et al., 1974; Munro et al., 2001; Oprian and Coon, 1982). In contrast, the reduction of P450 is by electron transfer from the fully reduced FMN. During steady‐state turnover the enzyme cycles predominantly between the one‐ and three‐electron reduced states (Fig. 5). In this catalytic cycle, the low‐level reactivity of a neutral (blue) FMN semiquinone with electron acceptors enables one‐electron transfer, and the FMN shuttles between the neutral semiquinone and fully reduced states. The first and second electrons from the reductase to P450 are sequentially transferred from the fully reduced states (V and IX) of FMN, which can donate an electron at constant oxidation‐reduction potential. This model could apply to that of the NOS reductase domain (Guan and Iyanagi, 2003; Guan et al., 2003). It is likely that the state, VI (FAD‐FMNH ) is a common predominant intermediate in the catalytic cycle, and the V and IX states can donate electrons to electron acceptors, including P450 (Garcin et al., 2004; Yamamoto et al., 2005).

_

_

_

b. Electron Transfer from P450R to P450 The three‐dimensional (3‐D) structures of P450R (Wang et al., 1997) and nNOS reductase domain (Garcin et al., 2004) indicate that the dimethylbenzene edge of the isoalloxazine ring of FMN, which is exposed in the FMN domain, is covered by FAD (Fig. 2). The pyrimidine ring of the FMN isoalloxazine is slightly buried by two loops, while the dimethylbenzene edge is exposed to solvent. There are several possible mechanisms for electron transfer from the FAD–FMN pair to the electron acceptor, including P450 and cytochrome c. Electron transfer from the FMN to

48

TAKASHI IYANAGI

FIG. 5

Reaction mechanism of P450R.

the electron acceptor could occur without an associated conformational change (Nikfarjam et al., 2006; Shen and Strobel, 1994), or with a large scale movement of the FMN domain (Auchus et al., 1998; Iyanagi, 2005a,b). The former model infers that electron transfer involves the pyrimidine ring. In this case, an electron tunneling pathway is presumably involved because the pyrimidine ring is buried in the protein. The aromatic amino acids, which sandwich the isoalloxazine ring of the FMN moiety, may participate in electron tunneling during transfer to the electron acceptor (Fig. 3). In this case, domain movement is not necessary for electron transfer. Alternatively, the fully reduced FMN may transfer electrons to P450 by interaction between the P450 and the FMN‐binding domain. This interaction may occur at the same structural region of the FAD‐binding domain (Auchus et al., 1998). Therefore domain movement may be needed to facilitate relative domain‐domain reorientation during the electron transfer process. Intramolecular one‐electron transfer from the reduced FAD to FMN occurs directly at the closest distance, as described previously. The dimethylbenzene ring of the FMN moiety must be positioned adjacent to the P450, which could be facilitated by a flexible linker between the FMN domain and the remainder of the molecule. Intriguingly, the isolated FAD domains of P450R and NOSs do not significantly reduce the isolated CaM‐bound FMN domains (Iyanagi, unpublished data). This observation suggests that the electrostatic interaction between FAD and FMN domains is less specific, indicating flexibility in the relative orientation between electron donors and electron acceptors during the catalytic cycle. Furthermore, crystal structures of wild‐type and various mutant P450Rs strongly suggest that the relative orientation and position of two flavin domains with respect to each other is quite flexible (Hubbard et al., 2001).

PHASES I AND II DRUG‐METABOLIZING ENZYMES

49

The interaction surface of a P450 is not well understood, but mutagenesis experiments indicate that P450R interacts with the proximal surface of P4502B4 (Bridges et al., 1998). The proximal surface, which contains the C‐helix and adjacent to the heme prosthetic group, is highly conserved in the residues from various P450, and relatively electron positive when compared with the distal surface (Bridges et al., 1998; Williams et al., 2000; Zhang et al., 2005; Zhao et al., 2006). This electropositive region may interact with the negative‐charged surfaces of FMN domain of P450R and/or b5, facilitating association and electron transfer (Allorge et al., 2005; Bridges et al., 1998; Scott et al., 2004; Zhao et al., 2006). The electrons from P450R might be transferred from the FMN of the reductase by interacting at the opposite side of P450 with respect to the membrane (see Fig. 12). The FMN‐binding domain interacts with P450 to transfer electrons during catalysis. Therefore, mutations in the FMN‐binding domain of P450R aVect the interaction with P450. The electrostatic potential surface of the FMN domain of P450R shows distinct regions of positive and negative charge, which results in a significant electrical polarity. The negative charge is located in the area of the FMN‐binding site. Zhao et al. (1999) carried out mutation analysis and demonstrated the importance of the electrostatic interactions involved in the binding of P450R to P450, including cytochrome c. The mutation D148N aVected several acidic residues near the FMN molecule. The results suggest that P450 binds at the tip of P450R to cover the FMN cofactor. This hypothesis is also supported by the fact that the much larger P450 molecule cannot fit into the crystal structure of P450R (Wang et al., 1997). The P4502D6*31 (CYP2D6) alleles are characterized by mutations encoding three amino acid substitutions: R296C, R440H, and S486T, although the R440H exchange alone is the inactivating mutation. The docking model between this mutant and P450R suggest that R440 constitutes part of a cluster of basic amino acid residues that play a role in P450R binding (Allorge et al., 2005). Jenkins et al. (1997) have shown that substitution (E154Q) in the corresponding acidic cluster of Anabaena flavodoxin aVects its ability to transfer electrons to P450c17 (P45017A1). The flavoprotein component of the Escherichia coli sulfite reductase can act as a mammalian P45017A1 reductase. These data indicate that plant and bacterial flavodoxin, including flavodoxin‐like domains, can donate electrons to mammalian P450. The mutation Q153R in human P450R (rat Q150), located at the FMN‐binding site, reduces the activity of P45017A1 and cytochrome c. P45017A1 is located on the ER of steroidogenic tissues, and catalyzes the hydroxylation of the steroid 17a. The B. megaterium P450BM3 fatty acid monooxygenase system is considered the best model system for understanding P450R–P450 interactions (Sevrioukova et al., 1999). However, this system operates as a dimer, and the P450 may accept electrons from the FMN of the reductase domain located on

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TAKASHI IYANAGI

the polypeptide partner (Neeli et al., 2005). Therefore, intramolecular electron transfer from FMN to heme may not occur. NOS also functions as a dimer in which the P450‐like domain accepts electrons from the FMN of the reductase domain located on the polypeptide partner (Garcin et al., 2004) (Figs. 1, 2). In the bacterial system, the flavodoxins can shuttle between the semiquinone and fully reduced states during the catalytic cycle (Nogues et al., 2005). In P450R, the fully reduced FMN states (V and IX) may be the open form in which they can transfer electrons to an electron acceptor (Fig. 6). States I, II, III, IV, VI, VII, and VIII are closed forms in which intramolecular electron transfer between flavins occurs (Iyanagi, 2005a,b). However, it is diYcult for the P450 and cytochrome c to gain access to the active site of these states. Therefore, the latter model assumes that intramolecular electron transfer between flavins is linked to a significant movement of the FAD domain. This model involves a redox‐linked conformational change during electron transfer (Figs. 5, 6). The electron acceptors accept an electron from FMNH2, whereas FMNH is an inactive intermediate observed during the catalytic cycle. Therefore, the initial reaction in the catalytic cycle starts from the air‐stable semiquinone species VI, and the V and IX states are active species for electron acceptors. With cytochrome c as the electron acceptor, a diVerent molecule accepts electrons independently from these states. In contrast, a P450 requires two electrons delivered in two one‐electron transfer steps. The same P450, which accepts the first electron from state V has to either move away from the reductase and accept an electron from a diVerent reductase molecule or interact with a diVerent site of the reductase (states VI, VII, VIII). This is followed by a redox‐dependent conformational change, where a second electron is accepted from state IX. The second electron is also supplied from b5, although the role of this transfer depends on the P450 isozyme, the substrate, and the precise experimental conditions (Zhang et al., 2005). These findings indicate that the proximal surface involved in the

_

FIG. 6 The proposed model for closed (A) and open (B) forms of P450R. The P450R might be in redox‐linked dynamic equilibrium between the closed and open forms (Iyanagi, 2005a,b).

PHASES I AND II DRUG‐METABOLIZING ENZYMES

51

interaction with P450R or b5 are either identical or partially overlapping. Therefore, when the P450 interacts with b5, the reductase must be displaced from the P450.

c. Activation of Molecular Oxygen by P450 The prokaryotic and eukaryotic P450s exhibit a conserved secondary structure and folding pattern (Mestres, 2005), and possess a common thiolate anion as the axial ligand of the heme (Omura, 2005). In the substrate‐binding cavity, molecular oxygen (O2) is activated by sequential one‐electron reduction of heme iron (Fig. 7). The first step involves substrate binding, resulting in a substrate‐bound form in equilibrium between high‐ and low‐spin states. Substrate binding causes a change of redox potential, which facilitates the initial reduction of substrate‐ bound P450 by the reductase (Sligar et al., 1979). The introduction of the first electron involves the reduction of ferric P450 (Fe3þ) and binding of O2. The second electron addition enables the heterolytic O‐O bond scission, in which the thiolate axial ligand of P450 promotes the cleavage of heme‐bonded dioxygen by increasing the electron density of the iron atom (Denosov et al., 2005; Hlavica, 2004). This reaction is coupled with proton donation. The 3‐D structure of the oxygenated form of P450eryF (Nagano et al., 2005) and P450CAM (Nagano and Poulos, 2005) supports the idea that the proton is supplied from a hydrogen‐bonding network including water molecule(s), forming the water and the ferryl, Fe4þ ¼ O species. This active motif, O ¼ Fe4þ S can act as an electrophilic oxidant (Groves, 2006). The oxygen of the ferryl species may be transferred to either a

FIG. 7 The role of first and second electrons for molecular oxygen activation by P450. The first and second electrons are supplied from FMNH2 of the P450R. In the NOS (Stuehr et al., 2005), the hydroxylated Arg (ArgOH) formed in the first turnover is further oxidized by a second turnover cycle, resulting in the formation of L‐citrulline (L‐Cit) and nitric oxide (NO). RH indicates substrate, and the S indicates the axial ligand, thiolate anion from cysteine.

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TAKASHI IYANAGI

carbon‐hydrogen bond (C‐H) (hydroxylase), bond (epoxidation), and heteroatom, such as a nitrogen or sulfur atom (hetero atom oxidation). Thus, the active oxygen‐transferring species, assumed to hydroxylate the substrate, may be formed by a concerted cleavage in a ‘‘push and pull’’ eVect mediated via the thiolate axial ligand and proton donation (Yoshioka et al., 2002). The strong axial electron donation to the iron center allows hydrogen atoms to be abstracted from R‐H bonds by ferryl radicals. It has been proposed that the hydroxylation reaction proceeds during the abstraction of a hydrogen atom from the substrate (RH), and one oxygen atom rebound as shown in Eqs. 2 and 3. RH þ O ¼ Fe4þ

.

R þ ðHO‐Feþ4

S S

.

! R þ ðHO‐Feþ4

S

Þ ! R : OH þ Feþ3

S

Þ

ð2Þ ð3Þ

The hydroxylation mechanism, including the hydrogen transfer (Eq. 2) and oxygen rebound (Eq. 3), appears to be the predominant mechanism (Groves, 2006). Bach and Dmitrenko (2006) proposed a modified mechanism in which the isomeric metastable hydroperoxide intermediate, OH. . .O‐Fe3þ S , which is formed from HOO‐Fe3þ S , is the primary oxidant in the hydrocarbon reaction. Furthermore, electron transfer to generate a carbocation followed by capture of a hydroxyl anion has been proposed as an alternative oxygenating principle (Ullrich, 2003). The NOS has been shown to catalyze a P450‐like reaction (McMillan et al., 1992), and converts L‐Arg into L‐Cit and NO in two consecutive reaction cycles with the intermediate formation of No hydroxy‐L‐arginine (ArgOH) within the same substrate‐binding site (Stuehr et al., 2005). In the first reaction, H4B serves as a transient one‐electron donor to the ferrous oxy‐ heme complex, because the radical form can accept one electron from the reductase, but the role of H4B in the second reaction is unknown. These reactions occur inside a dimeric complex enzyme, in which the first and second electrons are supplied from FMNH2 of the reductase located on the other subunit (Fig. 1). Likewise, because the P450R/P450 system is composed of distinct protein components, these reactions also occur by interaction between two diVerent molecules. In both systems, thiol ligation to the heme iron enables the formation of the Fe4þ ¼ O species and oxygen transfer to substrates by sequential electron transfer from a reductase, containing FAD and FMN (Fig. 7). d. Regulation of FAD‐FMN Pair in P450R and NOS Reductase Domain Electron transfer between most reactants in a biological system occurs between spatially fixed and oriented sites. A theory by Marcus and Sutin (1985) introduces a steric factor S for the intramolecular electron transfer, which takes into account the restricted orientation of donor (D) and acceptor (A)

53

PHASES I AND II DRUG‐METABOLIZING ENZYMES

at a distance appropriate for electron transfer in protein systems. The reaction between D and A proceeds as follows:

D þ A ! D A!D A!Dþ ! Dþ A !Dþ þ A

A

ð4Þ

where D A and D A represent the encounter complex and the active electron transfer complex, respectively. The D A complex is formed from the encounter complex D A by suitable reorientation of D and/or A. The distance between D and A is regulated by the dynamics of the conformational changes in the complex. The electron transfer rate constant (ket) is largely dependent on the separation distance between the electron donor and acceptor, and the redox potential diVerence, G0, between the donor and acceptor sites. These processes include at least three elemental steps: (1) formation of an active donor–acceptor complex; (2) electron transfer between the donor and acceptor; and (3) dissociation of the oxidized and reduced products. In the FAD–FMN pair of P450R and NOS isoforms, electron transfer occurs from FAD (donor) to FMN (acceptor). The active complex (FAD–FMN) is formed between the FAD and FMN molecules and electron transfer takes place directly between these flavins (Fig. 3). Although the FAD–FMN pair of P450R is not strictly regulated, the reductase domains of nNOS and eNOS are regulated by CaM‐binding. In contrast, the iNOS isozyme, which can bind CaM tightly at physiological concentrations of Ca2þ, is already in the activated form. Comparison of NOS reductase with P450R shows it to contain additional regulatory loops that control enzyme activity (Fig. 2). Regulation of nNOS and eNOS is achieved by the reversible binding of CaM to the inter‐domain hinge region brought about by changes to the intracellular level of Ca2þ. Binding of CaM activates electron transfer from FMN to heme, resulting in the turnover of L‐Arg and oxygen at the heme site. Interestingly, the isolated reductase domain of nNOS and eNOS is also activated by CaM. Cytochrome c, which can act as an artificial electron acceptor, is able to accept an electron from FMN of the nNOS reductase domain in the absence of CaM, but its rate of electron transfer is significantly accelerated (20‐fold) in the presence of CaM (Guan and Iyanagi, 2003; Guan et al., 2003; Matsuda and Iyanagi, 1999). In contrast, the reduction of ferricyanide, which mainly accepts electrons from FAD, is activated only two‐ to fivefold by the binding of CaM. The data strongly suggest that either the reduction of FAD or interflavin electron transfer between FAD and FMN are activated by binding of CaM. As suggested from the position of the AI motif and C‐terminal a‐helix (Fig. 2), CaM binding might participate in increasing the eYciency of electron transfer by adjusting the distance and orientation between the FAD and FMN cofactors. Another model for the activation of the cytochrome c reductase activity suggests

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that conversion from the CaM‐free closed form to the CaM‐bound open form is controlled by the binding of CaM (Craig et al., 2002). In this model, cytochrome c can react with the CaM‐bound open form. However, the conformational change induced by CaM‐binding is not absolute, because the reduction of the flavins is increased by CaM‐binding (Guan and Iyanagi, 2003; Guan et al., 2003; Matsuda and Iyanagi, 1999). Both mechanisms may be involved in the activation of cytochrome c reductase activity. The crystal structure of a CaM‐free nNOS reductase domain revealed an ionic interaction between Arg 1400 in the C‐terminal tail regulatory element and the 20 ‐phosphate group of bound NAD(P)H. Mutations of this residue (Arg1400Ser or Glu) increase cytochrome c reductase activity, indicating destabilization of a ‘‘shielded’’ conformation for the FMN module. However, no NO synthesis can be detected in the CaM‐free state. These reports indicate that additional structural changes induced by the binding of CaM allow an interaction of the FMN module and the oxygenase heme domain to facilitate eYcient electron transfer (Tiso et al., 2005). Roman et al. (2000) reported about 30 amino acids from the C‐terminal region of NOS repress enzyme activity in the absence of CaM. C‐terminal deletion mutants possess increased cytochrome c activity in the absence of CaM, as well as displaying NO synthase activity. Roman et al. (2000) also suggested that this tail region, which is located between the flavins and/or between FAD and NADPH (Garcin et al., 2004), might aVect interflavin electron transfer in NOS (Jachymova et al., 2005). The turnover numbers for NO synthesis catalyzed by the isoforms of NOS have been determined as 200 min 1 for iNOS, 100 min 1 for nNOS, and 20 min 1 for eNOS (Roman et al., 2002). The overall rate‐limiting step in the NOS system is the reductase domain and heme center. An increase in flavin domain activity increases NO synthase activity (Nishida and de Montellano, 1998), indicating the diVerent regulation by CaM of the reductase domain in the NOS isoenzymes. It is interesting to speculate whether interflavin electron transfer or dynamic equilibrium between the closed (shielded) and open (deshielded) forms might be diVerentially controlled. Both reductase domains have a diVerent activity for ferricyanide and cytochrome c. Ferricyanide activity for both enzymes is greater than of cytochrome c. The cytochrome c activity for eNOS is lower than for nNOS, which correlates with the interflavin electron transfer in the two isoforms (Nishino et al., 2003). Moreover, the extent of activation of eNOS by CaM is lower than of nNOS. Therefore, activation of the nNOS and eNOS isoforms by CaM might involve both (1) activation of the reductase domain, including electron transfer between flavins, accompanied by conformational change (Craig et al., 2002; Iyanagi, 2005a,b; Matsuda and Iyanagi, 1999), and (2) interaction between the FMN module and heme domain accompanied by conformational change (Feng et al., 2006; Garcin et al., 2004; Roman and Masters, 2006). Thus, an electron transfer

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may be directly linked to a change in conformation, which is diVerentially controlled in the nNOS and eNOS isoforms.

C. Antley‐Bixler Syndrome/Missense Mutations of P450R Although there are numerous functional cytochrome P450 genes in mammals, there is only one P450R gene in each species. Thus a single P450R is responsible for electron transfer to all the microsomal P450s. Knocking out the P450R gene in mice leads to embryonic lethality (Otto et al., 2003; Shen et al., 2002), and missense mutations of the human P450R gene cause multiple steroidogenic defects and a skeletal dysplasia called Antley‐Bixler syndrome (Adachi et al., 2004; Arlt et al., 2004; Fluck et al., 2004; Huang et al., 2005a; Miller, 2005). The P450R missense mutations could aVect the reduction of microsomal P450 enzymes involved in the biosynthesis of steroids by several diVerent mechanisms. For example, mutations in P450R may interfere with: (1) cofactor binding (NADP(H), FAD or FMN), (2) hydride transfer from NADPH to FAD, 3) interflavin electron transfer between FAD and FMN, or (4) interaction of P450R with P450 (Figs. 5, 6). This syndrome is also caused by disorders of steroidogenic P450s, which accept electrons from microsomal or mitochondrial P450‐containing electron transfer systems (Fig. 1). Intriguingly, the mutations in P450R that give rise to Antley‐Bixler syndrome might also have parallels with mutations aVecting the NOS reductase domains. Such mutations are likely to cause disorders in neuronal transmission, the immune system, and control of vascular wall functions. The Shen and Kasper group (1989, 1991, 1995, 1996, 1999, 2000) have used site‐specific mutation analysis to probe important amino acid residues involved in catalysis. Huang et al. (2005a) have analyzed the mutations in P450R in patients with Antley‐Bixler syndrome by using reconstituted system. Several missense mutants of human P450R (Y181D, R616X, R457H, Y459H, V492E) result in low activities of cytochrome c, 17a‐hydroxylase, and 17,20 lyase. However, the mutations Q153R, L565P, C569Y, and V608F result in only a mild impairment of these electron acceptors. The isoalloxazine ring of FAD and FMN molecules are sandwiched between two aromatic groups (Fig. 3). The hydrogen bonding and van der Waals interactions between amino acid residues and the FAD and FMN cofactors serve to regulate both the binding and reactivity of the flavins. The Y140 residue, located on the re‐side, lies at an angle of 40 to the isoalloxazine ring, whereas the Y178 residue is parallel to the si‐side of the FMN ring. These two aromatic amino acid residues are involved in binding of FMN to the protein (Wang et al., 1997). To test this hypothesis, Shen et al. (1989) prepared rats carrying the P450R mutant Y178D (equivalent to human Y181). A lowering of the FMN levels in the Asp mutant reduced the cytochrome c reductase

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activity. These results are entirely consistent with the hypothesis that an aromatic residue at position 178 is required for binding of FMN (Fig. 3). The corresponding mutation in human P450R (Y181D) results in the anticipated enzyme defects. The FAD molecule is also sandwiched between two aromatic groups: W677 stacked against the re‐face, and Y456 positioned at an angle of 60 to the si‐face. This arrangement of aromatic residues is similar to that found in the FMN‐binding site (Fig. 3). Mutation of Y456, which hydrogen bonds to the ribityl 40 ‐hydroxyl moiety of the flavin, results in a drastic loss in aYnity for FAD (Shen and Kasper, 2000). The corresponding human Y459H (rat 456) mutation causes a decrease in the activity of enzymes associated with P450R. The negative charge of the pyrophosphate moiety of the FAD molecule is stabilized by the R454, V489, and T491 (Wang et al., 1997). Mutation of T491 has a relatively modest eVect on FAD‐binding compared with mutation of R454 (Shen and Kasper, 2000). The corresponding human R457H mutant (rat 454) and V492E (rat 489) results in a marked reduction of the activities associated with P450R (Adachi et al., 2004; Fluck et al., 2004; Huang et al., 2005a). Mutations of R457H and V492E cause a decrease in the FAD‐binding aYnity (Marohnic et al., 2006). Alkylation, using iodoacetic acid, of the conserved cysteine (C566) residue in P450R (Haniu et al., 1984; Shen et al., 1991), causes a decrease in enzyme activity. The cysteine residue is protected from alkylation by the presence of NADPH, indicating a role for C566 (corresponding to human C569) in the binding of NADPH. A mutation of C569Y in humans causes a disorder in steroidogenesis, suggesting that the insertion of a bulky amino acid residue (i.e., tyrosine) reduces binding of NADPH. However, mutations on the interflavin electron transfer between FAD and FMN, and interaction with P450 have not been identified.

III. Phase II: UDP‐Glucuronosyltransferase (UGT) Phase II conjugation reactions lead to the formation of a covalent linkage between a functional group either on the parent compound or on one introduced as a result of a phase I reaction. UDP‐glucuronosyltransferases (UGTs) are the major class of enzymes that catalyze phase II reactions, such as the transfer of glucuronic acid (GlcUA) of UDP‐glucuronic acid (UDP‐ GlcUA) to a functional group (‐OH, ‐SH, ‐NH2, C‐C, or ‐COOH) of a xenobiotic and endobiotic. The xenobiotic may be a drug molecule or an endobiotic, such as bilirubin, bile acid, thyroxin, biogenic amine, fat‐soluble vitamin, or steroid (Belanger, 2003; Bock, 2003; Clarke and Burchell, 1994; Guillemette et al., 2003; King et al., 2000; Mackenzie, 1990; Radominska‐Pandya et al.,

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1999; Siest et al., 1987; Tukey and Strassburg, 2000). The enzymes comprise a large superfamily that can be classified, based on the degree of amino acid similarity between isoforms, into four gene families (Burchell et al., 1991; Mackenzie et al., 1997, 2005; Owens et al., 2005). There are numerous functional UGT genes in mammals (i.e., 17 in rat, 18 in mouse, 19 in human). In this section, the structure/function of microsomal UGTs and their gene organizations are described.

A. Historical Perspective In 1959, Williams (Williams, 1959) proposed that drugs and foreign molecules are metabolized in two distinct phases (phases I and II). In the early 1950s, however, little was known about the UGT enzymes involved in the metabolism of xenobiotics and endobiotics. Dutton and Storey (1951, 1953) discovered a thermostable cofactor in liver required for the formation of a phenol glucuronide in a cell‐free preparation. They isolated and identified uridine diphosphate glucuronic acid (UDP‐GlcUA) and its components, including uridine, two phosphates, and GlcUA, by paper chromatography (Dutton and Storey, 1954; Storey and Dutton, 1955). It was suggested that UDP‐GlcUA may act as a GlcUA donor in the formation of glucuronides. Strominger and coworkers (1954, 1957) purified uridine diphosphate glucose dehydrogenase, which catalyzes the conversion of UDP‐glucose (UDP‐Glc) to UDP‐GlcUA. In 1954, Axelrod and Brodie (reflection by Axelrod, 2003) studied the formation of morphine glucuronide after incubating microsomes and the cytosolic fraction of rat liver with UDP‐Glc and either TPNþ (NADPþ) or DPNþ (NADþ). Morphine glucuronide was formed in the presence of DPNþ (NADþ). These pioneering experiments opened a new field into the enzymatic formation of glucuronide conjugates, including phase II reactions. Furthermore, these studies also led to the discovery of the role played by bilirubin glucuronide formation in jaundice. Analysis of the hereditary jaundiced Gunn rat (Axelrod et al., 1957; Gunn, 1938; Schmid et al., 1957) paved the way to understanding the human disease Crigler‐Najjar syndrome (Crigler and Najjar, 1952). In the 1950s–1960s, UDP‐GlcUA was established as the glucuronyl donor during the biosynthesis of glucuronide derivatives of esters, aliphatic/aromatic compounds, steroids and bilirubin. UDP‐GlcUA þ ROH ! UDP þ RO‐GlcUA

ð5Þ

In general, conjugation reactions result in the formation of water‐soluble, pharmacologically inactive metabolites. However, some biologically active or

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highly reactive conjugated metabolites can also be generated. For example, morphine‐6‐O‐glucuronide is a more highly analgesic substance than the parent compound in suppressing pain symptoms in humans (Shimomura et al., 1971; Yamada et al., 2003; Yoshimura et al., 1968). Furthermore, acyl‐GlcUA derivatives can be quite reactive, resulting in the transfer of GlcUA to albumin (Smith et al., 1989). UGTs are membrane‐bound enzymes with a markedly lower activity in native microsomes compared to disrupted microsomes. Two hypotheses, known as ‘‘compartmentalization’’ and ‘‘conformation,’’ were put forth to explain this observation. The former model proposed that the enzyme is located on the luminal side of the ER, with translocation of UDP‐GlcUA from the cytosol being a rate‐limiting step (Battaglia et al., 1996; Bossuyt and Blanckaert, 1997; Vanstapel and Blanckaert, 1988). In contrast, the latter model proposed that the enzyme is constrained by interactions between the protein and the membrane lipid bilayer (Vessey and Zakim, 1971; Zakim and Dannenberg, 1972). These models led to an understanding of the structural features of UGT as a membrane‐binding enzyme and the localization to the ER membrane. The purification and characterization of UGTs provided important information concerning the heterogeneity and properties of these enzymes. Isselbacher et al. (1962) partially purified the enzyme from rabbit liver microsomes after treatment with detergent. This pioneering work suggested the existence of more than one glucuronosyltransferase activity. Further purification of the enzyme was reported from many laboratories (Bock et al., 1979; Burchell, 1977; Ishii et al., 1993; Mackenzie et al., 1985; Weatherill and Burchell, 1980; Yokota et al., 1988). However, the isoforms of UGT were systematically separated from rat liver microsomes by chromatofocusing and aYnity chromatography (Falany and Tephly, 1983). This systematic study has resulted in significant advances in our understanding of the biochemistry of UGTs. In the mid 1980s, three groups (Iyanagi et al., 1986; Jackson and Burchell, 1986; Jackson et al., 1985; Mackenzie, 1986a,b; Mackenzie et al., 1984) isolated cDNA of UGTs. These studies have allowed the analysis of the gene structure and the detection of specific UGT isoforms in tissue samples and cell lines. Nagai et al. (1988) suggested that bilirubin and phenol UGT genes are closely linked on the same chromosome. In addition to bilirubin, the Gunn rat is also deficient in a 3‐methylcholanthrene‐inducible UGT isoform that has high activity toward phenolic substrates (Iyanagi et al., 1989). Indeed, these two genes were subsequently located on the UGT1 gene complex (Emi et al., 1995). The UGT genes are mainly encoded by the UGT1 gene complex locus, family 1 (Emi et al., 1995; Ritter et al., 1992; Zhang et al., 2004) and family 2 (Mackenzie and Rodbourn, 1990) genes.

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B. UGT 1. Structure and Function UGTs are a family of membrane‐bound enzymes that are concentrated in the ER and nuclear envelope of hepatocytes (Roy Chowdhury et al., 1985). The major part of the enzyme is orientated on the luminal side of ER where the catalytic site is located. Each UGT enzyme includes an amino‐terminal signal peptide that is cleaved during synthesis of the polypeptide chain and a stretch of 17 hydrophobic amino acids near the C‐terminus that anchors the protein to the lipid bilayer (Iyanagi et al., 1986) (Fig. 8). Indeed, the C‐terminal 20–30 amino acid residues are responsible for the retention of UGTs in the ER (Jackson et al., 1990; Teasdale and Jackson, 1996). The mammalian UGT gene superfamily can be divided into four families: UGT1, UGT2, UGT3, and UGT8 (Burchell et al., 1991; Mackenzie et al., 1997, 2005). Members of the UGT1A family share an identical C‐terminus (ca. 245 amino acids), which includes the binding site for the common

FIG. 8 Functional domains of microsomal‐ and Golgi‐type UGTs and plant GT. Microsomal‐ type UGT indicates rat UGT (Iyanagi et al., 1986). Golgi‐type UGT indicates human b1, 3‐glucuronosyltransferase 1(GlcAT‐I) (Pedersen et al., 2000). Plant GT indicates the UGT71G1 (Shao et al., 2005). SP, signal peptide; NBD, highly conserved nucleotide‐binding domain; TM, transmembrane domain; DxD, DxD motif. HVRI and HVRII indicate the hypervariable region I and II (Iyanagi, 1991), respectively. The N255 in the UGT71G1 is located in the loop linker between the N‐ and C‐terminal domains.

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cosubstrate UDP‐GlcUA, whereas the N‐terminal region (ca. 286 amino acids) shows a markedly lower level of identity (37–49%). The N‐terminal portion of the enzyme contains the substrate‐binding site and includes two hypervariable regions (Iyanagi, 1991) (Fig. 8). In contrast to the UGT1 family, the UGT2 family enzymes do not share a common C‐terminal domain. However, the human genome project suggests that UGT2A1 and UGT2A2 genes can share a common C‐terminal domain (Mackenzie et al., 2005). Comparison of members of the UGT2 gene family indicates that amino acid diVerences between diVerent isoforms occur throughout the length of the protein, although the C‐terminal halves are highly conserved. The proteoglycan‐associated b1,3‐glucuronyltransferase 1 (GlcAT‐I) and human natural killer‐1 (HNK‐1)–associated glucuronyltransferase (GlcAT‐P) are localized on the luminal side of the Golgi membrane and have a transmembrane and stem region at the N‐terminus (Kakuda et al., 2004; Negishi et al., 2003; Sugahara et al., 2003). The overall 3‐D structures of both enzymes are similar and comprise two subdomains—an N‐terminal subdomain containing the UDP‐GlcUA‐binding site and a C‐terminal subdomain for substrate binding. Although GlcAT‐I and GlcAT‐P catalyze the transfer GlcUA from UDP‐GlcUA to an acceptor sugar, they do not display any significant sequence homology with that of the microsomal UGTs. This indicates the existence of diVerent UDP‐glucuronosyltransferase families in the Golgi and ER membranes (Fig. 8). The 3‐D structure of GlcAT‐I and GlcAT‐P in the presence of both donor and/or acceptor substrate suggests that the inverting glycosyl transfer reaction proceeds through an SN2‐type in‐line displacement mechanism, which generates a b bond from the a‐linked nucleotide sugar. In both enzymes, a glutamate residue acts as a catalytic base that deprotonates the 3‐hydroxy of the terminal sugar in the acceptor substrate to form a strong nucleophile. The nucleophile then attacks the C‐1 carbon of GlcUA in the UDP‐GlcUA donor and forms an oxocarbenium ion‐like transition state, similar to that proposed for glycosidase reactions (Cetinbas et al., 2006). This results in the formation of a b1‐3 linkage and the subsequent dissociation of UGT (Kakuda et al., 2004; Negishi et al., 2003). A similar mechanism may be operating in microsomal UGTs (Radminska‐ Pandya et al., 1999), although the 3‐D structure of a microsomal enzyme has not been solved. Ouzzine et al. (2000) suggested that histidyl and aspartic/ glutamic acid residues are likely candidates as base catalysts in microsomal UGTs. Interestingly, H38 and H485 in the sequences of rat and human UGTs are critical for activity because mutation results in an inactive enzyme. The structures of plant UDP‐flavonoid/triterpene GT, UGT71G1 (Shao et al., 2005) and UDP‐glucose:flavonoid 3‐O‐glycosyltransferase, VuGT1 (OVen et al., 2006) suggest that the H22‐D121 (UGT71G1) and H20‐D119 (VuGT1) pairs can function as catalytic bases (Fig. 9), respectively. In contrast,

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A

B

UDP E281

D119 H22

UDP-Glc

FIG. 9 The structures of GT‐A fold (A) and GT‐B fold (B). A, b1,3‐glucuronosyltransferase I (GlcAT‐I) (PDB code 1FGG). B, UDP‐flavonoid/triterpene GT, UGT71G1 (PDB code 2ACW).

the E281 in the GlcAT‐I (Negishi et al., 2003; Pedersen et al., 2000) and E284 in the GlcAT‐P (Kakuda et al., 2004) can function as catalytic bases. 2. Gene Organization The organization of the UGT1 gene complex is unique among the genes involved in the metabolism of druglike molecules. The UGT1 isoforms are generated by alternative splicing of the transcript. The 50 ‐exon genes of the UGT1 family each contain a unique first exon, plus four exons shared between the genes (Fig. 10A). The first exons appear to have evolved by a process of duplication, leading to the synthesis of proteins with identical C‐terminal (constant exon) and variable N‐terminal domains (variable exons) in human (Gong et al., 2001; Owens et al., 2005; Ritter et al., 1992), rat (Emi et al., 1995; Iyanagi, 1991) and mouse (Zhang et al., 2004). The human UGT1 gene complex is located on chromosome 2(2q37). Thus the C‐terminal domain of UGT1 family is responsible for the function of all UGT1 isoforms. Therefore, the mutations of this domain may lead to defects of multiple UGT1 enzymes (Iyanagi, 1991). In contrast, the human UGT2 genes are clustered on chromosome 4q13– 4q21.1 (Turgeon et al., 2000). Exon‐sharing is also seen with the six‐exon UGT2A1 and UGT2A2 genes. However, UGT2A3 and those of the UGT2B (six exons), UGT3 (seven exons), and UGT8 gene families (five or six exons) do not share exons and are probably derived by a process of duplication of all exons in the gene (Mackenzie et al., 1997, 2005; Turgeon et al., 2000). Analysis of the C‐terminal domain of the UGT1 and UGT2 families indicates a high degree of sequence conservation to accommodate a common UDP‐ GlcUA‐binding site. Most UGT1 and UGT8 enzymes have been characterized

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FIG. 10 The UGT1 gene complex and UGT2 family genes (A), and other complex genes (B). (A) The human UGT1 gene complex contains at least 13 variable exons, A1–A13 (Gong et al., 2001; Mackenzie et al., 2005), which can be spliced to constant exons, II–V. The variable exons are named A1, A2, A3. . ., and their gene products UGT1A1, UGT1A2, UGT1A3, etc. The human UGT1 and UGT2 loci extended over approximately 200 kb and 1.45 Mb, respectively. Pseudogene names end in the label P. The exons are not drawn to scale. (B) Complex gene locus for human immunoglobulin heavy chain (IGH), human protocadherins (PCDH) (Zhang et al., 2004) and human b1,6‐N‐acetylglucosaminyltransferase (Inaba et al., 2003; Yu et al., 2003).

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in detail, although the catalytic functions of the UGT3A enzymes and several UGT2 enzymes remain to be investigated (Mackenzie et al., 2005). The expression of specific UGT1 isoforms is achieved by selective activation of promoters preceding each variable exon (Emi et al., 1995; Owens et al., 2005; Sugatani et al., 2005; Usui et al., 2006). The UGT2 isoforms are also regulated by the promoter of each gene (Gardner‐Stephen et al., 2005; Mackenzie et al., 2003). There is compelling evidence that the expression of the mouse, rat, and human UGT1 and UGT2 genes are regulated in a tissue‐ specific manner (Bock, 2003; Bock and Kohle, 2005; Chen et al., 2005; Emi et al., 1995, 1996, 2005; Gardner‐Stephen et al., 2005; Leung and Ho, 2002; Mackenzie et al., 2003; Owen et al., 2005; Shelby et al., 2003; Tukey and Strassburg, 2000; Zhang et al., 2004). The UGT1 gene is found in several animal species, including mouse (Zhang et al., 2004), rat (Emi et al., 1995), rabbit (Lamb et al., 1994), monkey (Albert et al., 1999), and human (Gong et al., 2001; Ritter et al., 1992). The arrangement of genes akin to the UGT1 complex is not observed for other drug‐metabolizing activities, including phase I, II, and III enzymes. However, a similar gene organization is found for protocadherin, a diverse group of genes encoding cell surface proteins with an N‐terminal cadherin‐like extracellular domain (Wu and Maniatis, 1999). The protocadherin genes are organized into three sequentially linked clusters, designated a, b, and g (Fig. 10B). The gene cluster consists of tandemly arrayed variable exons, which encode an extracellular domain consisting of six cadherin‐like ectodomain repeats, a transmembrane domain, and a short cytoplasmic tail. At the 30 end of both the a and g subclusters are an additional three short exons that are alternatively cis‐spliced to each a and g variable exon, providing a constant cytoplasmic region. This gene cluster has been reported in zebrafish, mouse, rat, chimpanzee, and human (Hirayama and Yagi, 2006; Wu, 2005). As for the UGT1 gene cluster, the protocadherin genes are expressed in a tissue‐specific manner with each variable gene preceded by a distinct promoter (Zhang et al., 2004). Although the splicing of the protocadherin variable exon to the constant exons is not fully understood, the mechanism is likely be the same as for the UGT1A gene complex. The DNA rearrangement and somatic substitution do not occur in this gene complex (Hirayama and Yagi, 2006). This precise cis‐ alternative splicing may be achieved by the tight coupling of transcription to translation (Maniatis and Reed, 2002). Furthermore, the I‐branching b‐1,6‐N‐ acetylglucosaminyltransferase (b1,6GlcNAcT) proteins are a family of type II transmembrane proteins, with the three isoforms encoded by genes similar to those of UGT1 and protocadherin (Inaba et al., 2003; Yu et al., 2003) (Fig. 10B).

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3. Evolutionary Aspects The bacterial and plant glycosyltransferases (GTs) are involved in cell wall and secondary metabolite biosynthesis. In plants, the glycosylation of small‐ molecular‐weight lipophilic acceptors is thought to be involved in a key mechanism of metabolic homeostasis. UDP‐Glc is the major activated sugar donor, although some isoforms use UDP‐GlcUA instead (Bowles et al., 2005; Li et al., 2001; Sawada et al., 2005). The P450s and GTs are involved in the biosynthesis of secondary metabolites. Although the P450R/ P450 system has a similar cellular organization to the mammalian system, most plant GTs are soluble enzymes. The GTs can function to increase the stability and solubility of secondary metabolites as well as facilitating their detoxification (Bowles et al., 2005, 2006). For example, the P450s and GTs are involved in the biosynthesis of glucosinolates, in which the toxic thiohydroximate is formed. The glycosylation of this compound can be considered as a detoxification reaction. The structures of GTs have been studied in bacterial, plant, and mammalian species. Interestingly, the majority of GTs belong to only two structural superfamilies—GT‐A and GT‐B folds (Bourne and Henrissat, 2001; Hu and Walker, 2002; Unligil and Rini, 2000)—and utilize an activated UDP‐ sugar as a donor. The GT‐A comprises two dissimilar domains (Fig. 9): an N‐terminal subdomain with a Rossman fold, which includes the donor UDP‐sugar‐binding site, and a C‐terminal subdomain composed mainly of mixed b sheets to which the acceptor sugar binds. The diversity of the acceptors is relatively low. The structure of human GlcAT‐I and GlcAT‐P shares this fold (Breton et al., 2006; Kakuda et al., 2004; Negishi et al., 2003), whereas the GT‐B superfamily is remarkably diverse although they possess a highly conserved two‐domain architecture (Figs. 8, 9). The typical GT‐B fold has been found in various glycosyltransferases (Breton et al., 2006): phage T4 DNA‐glucosyltransferase (BGT), which attaches glucose to hydroxymethyl cytosines on the DNA duplex; E. coli MurG, a glycosyltransferase that catalyzes the transfer of N‐acetylglucosamine from UDP to the C‐4 position of a lipid‐linked N‐acetylmuramyl peptide acceptor; bacterial vancomycin UDP‐glycosyltransferases (Gtfs), which attach a glucose unit to a hydroxyl moiety; and plant UDP‐flavonoid/triterpene GT, UGT71G1 and UDP‐glucose:flavonoid 3‐O‐glycosyltransferase, VuGT1, which are involved in the biosynthesis of saponins and anthocyanins. These enzymes contain two a/b open sheet domains separated by a deep cleft. Structural analysis suggests that the C‐terminal domain contains the UDP‐GlcNAc‐binding site, whereas the N‐terminal domain contains the acceptor’s (substrate’s)‐binding site. The structures of these enzymes are characterized by two similar Rossman fold subdomain. Sequence alignments of GT‐B superfamily members reveal a conserved motif that corresponds to the a/b/a fold, composed of about 30

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amino acid residues, in the C‐terminal domain of BGT and MurG (Ha et al., 2000; Hu and Walker, 2002; Kapitonov and Yu, 1999). The microsomal UGT isoforms (Clarke and Burchell, 1994; Mackenzie, 1990; Mackenzie et al., 1997; Radominska‐Pandya et al., 1999) also possess this consensus sequence in the UDP‐GlcUA‐binding site (Fig. 8). This sequence is conserved in plant GTs (Gachon et al., 2005). It is likely that the microsomal UGTs belong to the GT‐ B family. In contrast, Golgi‐type UGTs contain the conserved DXD motif, which interacts with the ribose of the UDP moiety of UDP‐GlcUA, as well as with the catalytically required divalent cation (Negishi et al., 2003). In addition to the bacterial enzymes, plant UDP flavonoid/triterpene GT (UGT71G1) also belongs to the GT‐B fold (Shao et al., 2005) (Fig. 9). Indeed, the structure of UGT71G1 is superimposable on bacterial GtfD despite the low level of sequence identity (10%). The greatest diVerence between the two enzymes is observed in the N‐terminal domain (residues, 155–210), which forms one side of the substrate’s (acceptor molecule’s) binding pocket. The C‐terminal domains of UGT71G1 and GtfD share a greater level of sequence similarity because they bind similar nucleotide sugar donor molecules in contrast to the N‐terminal domains, which recognize quite diVerent acceptor molecules. Indeed, a conserved steroid‐binding sequence has been identified in the N‐terminal domain of plant GT isoforms (Kohara et al., 2005; Moehs et al., 1997). No microsomal UGT crystal structure is available, but structures of GT‐B fold family proteins from diVerent species suggest that mammalian microsomal UGTs might be composed of two subdomains. Microsomal UDP‐galactose:ceramide galactosyltransferase (CGT), which transfers galactose to lipophilic ceramide, belongs to family 8 (Ichikawa et al., 1996; Mackenzie et al., 2005) and is located in the ER membrane. The enzyme contains a nucleotide recognition domain which is located close to the C‐terminal end of the C‐terminal transmembrane domain. In contrast, plant diacylglycerol galactosyltransferase (DAGGalT), which catalyzes the synthesis of the major chloroplast membrane, is involved in the final step of peptidoglycan synthesis. This observation implies that the mechanism of chloroplast membrane biosynthesis is related to that of the bacteria cell wall. Although plant DAGGalT (Miege et al., 1999) and bacterial MurG (Ha et al., 2000) lack an identifiable terminal transmembrane domain, they are known to be membrane‐associated proteins. However, the greatest diVerence between mammalian UGTs and bacterial/plant GT‐B is in a C‐terminal transmembrane hydrophobic domain. This motif has not been reported in bacterial and plant GTs (Gachon et al., 2005). Taken together, the data strongly suggest that microsomal UGTs are evolutionarily related to GTs from bacteria and plants (Bock, 2003; Mackenzie et al., 1997). The structure of GT‐A fold and the N‐ and C‐terminal domains of GT‐B fold are similar to each other (Shao et al., 2005), although GT‐A fold enzymes contain only a single extended domain that recognizes both domain

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and acceptor. This suggests that GT‐A and GT‐B enzymes are evolutionarily related. The GT‐B enzymes, which are domain recognizing similar domains and another adapting divergent acceptors in the natural environment, might be produced as discussed in Fig. 11. One can speculate on the evolution of two domain enzymes, C‐V for GT‐A enzymes or V‐C for GT‐B enzyme, in which one domain recognizes similar nucleotide sugar donors (conserved domain, C) whereas the other has adapted to recognize diVerent acceptors (variable domain, V). The vertebrate enzymes have also acquired a membrane‐binding domain (Fig. 11). For example, the GT family of proteins from Caenorhabditis (C.) elegans contain a nucleotide sugar‐binding motif and a C‐terminal transmembrane domain and C‐terminal motif similar to the ER retention signal (Kapitonov and Yu, 1999; Mackenzie et al., 1997). These domains may have played an important role in the evolution of multicellular organisms. Fish, which are the most ancient vertebrates, contain multiple UGT isoforms with similar functional and structural properties to mammalian UGTs. This demonstrates a strong evolutionary conservation between phyla that diverged over 350 million year ago (Clarke et al., 1992a). Moreover, the zebrafish EST project did not provide any evidence for an elaboration of family 1A genes by alternative splicing of multiple exons (George and Taylor, 2002). Mammalian UGTs have developed the ability to accept diVerent substrates by forming a gene complex as well as duplicating gene clusters.

FIG. 11 A model for the evolution of domains in the microsomal UGT family 1 and 2 genes and Golgi GTs (UGTs) genes. C indicates the nucleotide‐sugar‐binding domain. V indicates the substrate‐binding domain. The number of human UGT1 and UGT2 isozymes, including pseudogenes is shown in parentheses. The putative transmembrane and the proposed nucleotide‐binding domains are indicated by bars (Fig. 8).

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The genomic ordering of variable exons of the UGT1 gene and their phylogenetic tree indicate that the UGT1A family can be broadly divided into two groups. The substrate specificity for UGT1A isoforms suggests that adaptive evolution has been involved in diversifying their functions. The variable exons are organized in a tandem array, so that a base substitution may result in gene conversion, as discussed for the protocadherin genes (Noonan et al., 2004). Interestingly, the two hypervariable regions in the UGT1 family are located at the N‐terminus (Iyanagi, 1991). Comparison of the UGT family members from several species shows that the C‐terminal domain is the most highly conserved region. It is likely that the C‐terminal domain was under evolutionary pressure to retain the binding site for the common UDP‐GlcUA substrate. The ratio of nonsynonymous (Ka) to synonymous mutations (Ks) in the conserved nucleotide‐binding segment of plant GTs is smaller than unity (Gachon et al., 2005).

C. Hyperbilirubinemia Bilirubin, the oxidative product of heme biotransformation in mammals, is a highly toxic compound that can cause severe brain damage in early childhood if allowed to accumulate in the body (Roy Chowdhury et al., 2001). The nonpolar characteristics of bilirubin allow the molecule to pass through the blood brain barrier. Bilirubin is excreted in bile after esterification with GlcUA to form polar mono‐ and diconjugated derivatives (Fig. 12). Accumulation of unconjugated bilirubin in the body is caused by hereditary disorders known as Crigler‐Najjar (CN) syndrome. The Gunn rat is a good model for unconjugated hyperbilirubinemia and valuable tool for the development of CN syndrome gene therapy. Severe hyperbilirubinemia may result from interaction with other mutated genes, such as glucose‐6‐phosphate dehydrogenase (Kaplan et al., 1997, 2003) and beta‐thalassemia (Sampietro et al., 1977). In addition to severe hyperbilirubinemia, single nucleotide polymorphism (SNP) in UGT family 1 enzymes can also cause a mild hyperbilirubinemia (Burchell, 2003; Guillemette et al., 2003; Koiwai et al., 1995; Mackenzie et al., 1997; Maitland et al., 2006; Owens and Ritter, 1992, 2005; Saeki et al., 2006). 1. Formation of Bilirubin Bilirubin is derived from the heme of hemoglobin and hepatic hemoproteins such as P450 and catalase, which contain the heme as a prosthetic group. The biotransformation of heme by heme oxygenase isoform I (HO‐1) proceeds in three successive oxygenation steps, via a‐meso‐hydroxyheme, verdoheme, and biliverdin. These reactions are catalyzed by microsomal HO‐I, which has a hydrophobic C‐terminus for binding to the microsomal membrane.

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The N‐terminal domain contains the heme‐binding site. Both molecular oxygen (O2) and NAD(P)H are required for the cleavage reaction, which proceeds via a multistep mechanism that depends on reducing equivalents provided by microsomal P450R (Colas and Ortiz de Montellano, 2003; Schacter et al., 1972). The two proteins are held together by electrostatic interactions between the positively charged HO‐I and negatively charged FMN‐binding site of P450R. Intriguingly, the aYnity of HO‐I for P450R increases upon addition of NAD(P)H (Higashimoto et al., 2005). It is likely that P450R combines with NAD(P)H to give the active conformation, which possesses a higher aYnity for HO‐I. The first step in the biotransformation of the heme group to bilirubin is the cleavage of its a‐methene bridge to form biliverdin IXa (Yoshida et al., 1981). The HO reaction starts with the formation of the ferric heme–HO complex which is reduced to a ferrous state by the first electron donated from P450R. Molecular oxygen then binds to the complex to form the oxygenated species. Upon receiving a second electron from P450R and a proton from the distal water pocket, the iron‐bound oxygen is converted to a hydroperoxide intermediate (Fe3þ‐OOH). The terminal oxygen of Fe3þ‐OOH attacks the a‐meso carbon of the porphyrin ring to form ferric a‐meso‐hydroxyheme (Davydov et al., 1999; Kikuchi et al., 2005). The hydroxylated compound is converted by two further oxidation steps to biliverdin IXa. The ultimate products of these reactions are biliverdin, iron, and carbon monoxide. The overall rate‐limiting step is in the release of biliverdin from the enzyme. The central methene bridge of biliverdin at C‐10 is then reduced by a cytosolic enzyme, NAD(P)H‐biliverdin reductase, to bilirubin. It is interesting to speculate whether the biliverdin reductase accepts biliverdin from the cytosol or directly from HO‐1. The release of biliverdin from HO‐1 is promoted by biliverdin reductase (Schuller et al., 1999), suggesting that HO‐1 interacts directly with biliverdin reductase to deliver biliverdin. The structure of HO‐1 indicates that half of the heme molecule is exposed to solvent. It has been proposed that biliverdin recognition by biliverdin reductase is achieved largely through an electrostatic interaction between the negatively charged propionate side chains of biliverdin and the positively charged residues of biliverdin reductase. Kikuchi et al. (2001) suggested that four basic residues of biliverdin reductase, located on the upper side of the putative NAD(P)H‐binding pocket, are important components of the interaction site. This pocket, which can accommodate both biliverdin and NAD(P)H, may accept biliverdin directly from HO‐1. Another possibility is that the liganding may mediate delivery of biliverdin from HO‐1 to biliverdin reductase. Bilirubin is an unsymmetrically substituted dicarboxylic acid. The introduction of CH2 at C‐10 induces a conformational change by rotation of the dipyrrinone groups about the central CH2 group. The conformational change promotes

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intramolecular hydrogen bonding of the propionic acid carbonyl to the amino groups of the dipyrrinone lactam and pyrrol ring. Indeed, these changes may explain some of the unusual properties of bilirubin, such as its high lipid/water partition coeYcient and resistance to hepatobiliary excretion (McDonagh and Lightner, 1985). Furthermore, the proposed conformation of bilirubin is extremely hydrophobic resulting in a high aYnity for tissues of the CNS. 2. Glucuronidation of Bilirubin and its Excretion in Bile The conjugated compounds with glucuronate, sulfate, or glutathione are substrates for organic anion uptake transporters in the basolateral (sinusoidal) membrane as well as substrates for the ATP‐driven conjugate eZux pump in the apical (canalicular) membrane, termed multidrug resistance protein 2 (MRP2; systematic name ABCC2) (Keppler, 2005). Bilirubin is a highly toxic and hydrophobic endobiotic. The oxidative biotransformation pathway from heme to bilirubin could be considered a phase I reaction, and its subsequent glucuronidation a phase II reaction (Fig. 12). Bilirubin, which is an organic anion with limited water solubility, is essentially unexcretable in its native form. Organic anion transport proteins, OATP2 (Kamisako et al., 2000; Konig et al., 1999) are involved in uptake of bilirubin from the plasma membrane. The UGT1A isoform, UGT1A1, in rats (Clarke et al., 1992b; Iyanagi, 1991) and humans (Bosma et al., 1994) have been implicated in bilirubin glucuronidation. The mechanism of uptake, modification, and excretion of bilirubin is thought to constitute a typical model system for the biotransformation of xenobiotics in vivo. The predicted topology of UGT on the ER membrane necessitates translocation of UDP‐GlcUA, which is synthesized in the cytosol, to the lumen of the ER. This step is thought to be rate‐limiting for UGT activity in the ER. Indeed, enzyme activity is increased upon disruption of vesicles with membrane‐ permeabilizing agents, such as detergent or alamethacin. UDP‐N‐acetylglucosamine (UDP‐GlcNAc) stimulates the internalization of UDP‐GlcUA into Reticuloendothelial

Hepatocytes

NADPH/O2 NADPH Heme

BV

P450R/HO

UDP-GlcUA

BIL BVR

BIL T

OATP2

ATP

BIL-GlcUA

UGT1A1

ADP

Bile MRP2

FIG. 12 Metabolic pathway from the heme group to bilirubin. P450R, NADPH‐cytochrome P450 reductase; HO, heme oxygenase; BV, biliverdin; BIL, bilirubin; BVR, biliverdin reductase; UGT1A1, UDP‐glucuronosyltransferase 1A1; OATP2, organic anion transporter 2; MRP2, multidrug resistance protein 2; T, proposed transporter.

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intact microsomal vesicles (Ikushiro et al., 1999). These observations strongly suggest the presence of transporters capable of delivering the UDP‐GlcUA from the cytosolic surface to the active site of the enzyme. Hauser et al. (1988) suggested that UDP‐GlcUA is transferred from the cytoplasm to the luminal side of ER by a specific transporter. Muraoka et al. (2001) discovered a novel human nucleotide sugar transporter, which transfers both UDP‐GlcUA and UDP‐N‐acetylgalactosamine (UDP‐GalNAc). The same transporter can participate in glucuronidation at the ER membrane and/or proteoglycan biosynthesis in the Golgi membrane. Microsomal UDP‐ galactose:ceramide galactosyltransferase (UGT8A1), which is found exclusively in the ER, forms a complex with the transporter for UDP‐Gal (Sprong et al., 2003). Although the transporter is confined to the Golgi, it can also be retained in the ER, allowing the formation of Gal‐ceramide. Furthermore, Csala et al. (2004) provide strong evidence for the presence of at least three diVerent glucuronide transporters in the ER membrane with partly overlapping substrate specificity. The data also indicate that the size and/or shape of the substrate, rather than the GlcUA moiety per se, is/are the important determinant(s) of transporter specificity (Battaglia and Gollan, 2001; Csala et al., 2004). In contrast, Ikushiro et al. (1997) suggested that the oligomer structures of UGTs might act as a common channel for the substrate and their conjugated products, although this does not require a specific transporter. The resulting bilirubin mono‐ and diglucuronides are then transported to the cytosolic side across the ER membranes and excreted into the bile by conjugate export pump, MRP2.

3. Hyperbilirubinemic Gunn Rat In 1938, Gunn (1938) described a mutant of Wistar rats (Gunn rats), which had hereditary hyperbilirubinemia. Homozygous Gunn rats are an excellent model of Crigler‐Najjar syndrome type 1, and have provided valuable information on bilirubin metabolism, bilirubin toxicity, treatment of hyperbilirubinemia, and the molecular mechanism of inherited jaundice. Defects of the UGT1 family in Gunn rats result in the formation of a common truncated C‐terminus. Therefore, all UGT1 isoforms are defective in the mutant rats, without aVecting the other UGT family (Iyanagi, 1991). This defect is caused by a 1 frameshift mutation, which generates a premature termination codon, resulting in truncated UGT1 proteins that lack the C‐terminal 116 amino acids (Emi et al., 1995; Iyanagi, 1991; Iyanagi et al., 1989). The truncated 43 kDa proteins, which have been detected in Gunn rat liver and kidney cells (ElAwady et al., 1990), are subject to rapid degradation by the proteasome (Emi et al., 2002).

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Therefore, Gunn rat has been a valuable model for investigating the eVect of multiple UGT1A enzymes in xenobiotic metabolism and toxicity (Kessler et al., 2002; Krishnaswamy et al., 2004; Narayanan et al., 2004). 4. Crigler‐Najjar Syndrome In 1952, Crigler‐Najjar described a syndrome characterized by a severe chronic nonhemolytic unconjugated hyperbilirubinemia (Crigler and Najjar, 1952). Two clinical forms of this syndrome have been described. The normal serum bilirubin levels are between 3–15 mM. Crigler‐Najjar (CN) syndrome type 1 patients have unconjugated serum bilirubin levels > 340 mM, whereas type 2 patients have levels ranging between 60–340 mM. Gilbert syndrome has levels < 60 mM (Burchell, 2003). The molecular basis of these syndromes has been characterized by genetic analysis. As a result of the elucidation of the hyperbilirubinemic Gunn rat and of the rat and human UGT1 gene complex, several groups have discovered the genetic lesions that cause hyperbilirubinemia. The mutations that result in CN syndrome type 1 (http://som.flinders.edu.au/ FUSO/ClinPharm/UGT/) have been found in the common exons and splicing sites as well as the first exon. Mutations in the first exon of UGT1A1, such as C280Stop(840C ! A), and G276R(826G ! C), indicate that human UGT1A1 is the major bilirubin isoform under physiological conditions (Bosma et al., 1994). CN type 2 and Gilbert syndrome are caused by mutations of both the first and common exons. Gilbert syndrome is also caused by a TA insertion in the TATA element (A [TA]6 TAA) in the promotor region of the first exon of UGT1A1 (Burchell, 2003). CN alleles are heterozygous in the coding region. The position of the mutation and its eVect on the activity toward bilirubin may determine the type of hyperbilirubinemia (Ciotti et al., 1999; Sugatani et al., 2001). 5. Gene Therapy Gene therapy is suitable for the most severe of the inherited defects of bilirubin conjugation, such as CN syndrome type 1. Treatment is based on the knowledge obtained for the rat and human UGT1 gene complex (Emi et al., 1995; Gong et al., 2001; Iyanagi, 1991; Ritter et al., 1992). As mentioned previously, the Gun rat is a good animal model for the molecular analysis of human hyperbilirubinemia. A major advantage of the Gunn rat is that the bilirubin glucuronides are not excreted into the bile. This allows direct and precise quantitation of the metabolic eVect of the transfer of a therapeutic gene. The Gunn rat has been used extensively for evaluating UGT1A1 gene transfer using diVerent vectors (Nguyen and Ferry, 2004) or oligonucleotide‐based gene therapies (Kren et al., 1999).

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Recombinant retroviruses and adenoviruses have been used for somatic gene therapy. For example, Takahashi et al. (1996) have used adenovirus vectors. When the recombinant vectors expressing human UGT1A1 were injected into newborn Gunn rats, the protein was predominantly detected in rat liver. However, the immune response was mainly directed against adenoviral protein. By contrast, Toietta et al. (2005) used helper‐dependent adenoviral vectors devoid of all viral coding sequence. Induction of prolonged transgene expression gave a significantly reduced chronic toxicity compared to early‐generation adenoviral vectors. The use of a tissue‐specific promoter, such as the rat phosphoenol‐pyruvate carboxykinase promoter, is also possible. Bellodi‐Privato et al. (2005) have used murine retroviral vector to treat neonate Gunn rats. The data indicate the liver is the main site of expression of the UGT1A1 protein, but there was also evidence of anti‐UGT1A1 antibodies in the rat serum. The third‐generation vectors, known as lentiviral vectors, have been used for safe, eYcient, and stable gene therapy in quiescent cells. This series of vectors, based on human immunodeficiency virus type 1 (HIV‐1), have been developed for the transduction of hepatocytes. Various in vivo promoters, such as human cytomegalovirus (CMV), human phosphoglycerate kinase, and the mouse albumin promoter, can be introduced into the HIV‐1–based vector. van der Wegen et al. (2006) used the lentiviral vector, which is under the control of the 1.9‐kb distal enhancer of the mouse albumin gene fused to 0.3 kb of the mouse albumin promoter. The human UGT1A1 protein was mainly expressed in the liver parenchymal cells. Nguyen et al. (2005) used the lentiviral vector under the control of a liver‐specific transthyretin promoter. Seppen et al. (2003, 2006) constructed a human UGT1A1 lentiviral expression vector under the control of a liver‐specific human phosphoglycerate kinase promoter, and found the recombinant protein expressed in several tissues. However, antibodies against UGT1A1 were detected in sera from rats injected during the fetal and neonatal period. These observations indicate that the xenogenic human UGT1A1 protein elicits a stronger immune response than endogenous rat UGT1A1. An alternative approach to using a gene transfer vector is the direct introduction of naked DNA into the target tissue (Danko et al., 2004). Jia and Danko (2005a) reported nonviral gene transfer of UGT1A1 using naked plasmid DNA injected into liver and muscle tissue. Expression was under the control of a CMV promoter. However, although repeat injections reduced serum bilirubin levels, the eVect did not exceed 2 weeks. Further studies to bring about more long‐term corrections are currently underway (Jia and Danko, 2005b). Kren et al. (1999, 2002) reported a novel method of gene therapy involving an in vivo site‐directed gene repair system. The technique relies on cellular DNA repair mechanisms to correct point mutations by using a synthetic

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RNA‐DNA chimera. The nucleotide sequence in the chimera is designed to be complementary to the target genomic sequence, except for a single mismatch. The mismatch between the DNA limb of the chimeric molecule and the complementary strand of the genomic DNA triggers the cell’s mismatch repair enzymes, resulting in correction of the mutation. For correction of the single guanosine base deletion in UGT1A1 exon 4 of the Gunn rat gene (Emi et al., 1995; Iyanagi, 1991; Iyanagi et al., 1989), the RNA‐DNA chain was constructed to contain the wild‐type sequence. The delivery system was targeted to the asialoglycoprotein receptor of hepatocytes. The presence of functional UGT1A1 protein was demonstrated by the appearance of bilirubin glucuronides in the bile and the concomitant reduction of serum bilirubin levels to 35–40% of pretreatment levels in Gunn rats. Furthermore, long‐term correction was observed at least 2 years after treatment. Experiments involving the gene therapy of Gunn rats have confirmed: (1) functional human UGT1A1 protein is expressed in the ER membrane of Gunn rat livers; (2) mono‐ and dibilirubin glucuronides are detected in bile; (3) a significant decrease of serum bilirubin levels can be elicited; (4) the UGT1A1 DNA is integrated in the chromosomal DNA; and (5) long‐term correction for UGT1A1 activity is also observed.

IV. Coordinated Biotransformation by P450 and UGT A. Subcellular Localization of the P450R/P450 System and UGT The cellular membrane consists of a bilayer of amphipathic lipid molecules, made up of a polar head group and a nonpolar hydrocarbon tail. The hydrophobic tails are buried within the bilayer whereas the hydrophilic head groups are exposed at the surface. All eukaryotic cells have an ER, which comprise a system of membranes that enclose a space, or lumen (Palade, 1956). The space or lumen is physically separated from the cytosol by the ER membrane, which mediates selective transfer of molecules between the two compartments. The ER is involved in the biosynthesis of cellular molecules, including proteins, carbohydrates, and lipids. In addition, the ER membrane plays an important role in the metabolism of druglike molecules. The typical phase I, P450R/P450 system is localized on the cytosolic side of the ER membrane, whereas the phase II, UGTs are localized on the luminal side (Fig. 13). Iyanagi et al. (1986), Mackenzie and Rodbourn (1990), Clarke and Burchell (1994), and Ishii et al. (2005) proposed a generally accepted model for the

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FIG. 13 The proposed model for topology of P450 reductase (FAD–FMN), P450 (Fe), UGT, and Transporters (T1 and T2) in the membrane of the ER. UGT is depicted as a dimer. T1 and T2 in the membrane of the ER represent the proposed transporters of UDP‐GlcUA (Muraoka et al., 2001) and glucuronides (Csala et al., 2004), respectively. UDP‐Glc, UDP‐ glucose; UDP‐GlcUA, UDP‐glucuronic acid; SULT, sulfotransferase; PAPS, 30 ‐phosphoadenosine 50 ‐phosphosulfate.

arrangement of the P450R/P450 system and UGTs in the ER membrane, although the biological significance of this orientation was unclear at the time. However, the given topology brings into question how the hydroxylated products of the P450s are delivered to the UGTs for further modification. Mammals possess numerous functional P450 genes (e.g., 84 in rat, 87 in mouse, 57 in human) (Gibbs et al., 2004) and UGT genes (e.g., 17 in rat, 18 in mouse, 19 in human) (Mackenzie et al., 2005). If the sequential reactions between P450s and UGTs occur on the ER membrane, approximately 103 possible combinations of human P450s and UGTs might occur (i.e., 50 microsomal P450s 19 UGTs). However, the number of functional combinations is restricted by the expression level and specificity for each isoform. The active site of microsomal P450s face toward the ER membrane from which the hydroxylated products can move to the cytosolic or luminal side of the membrane (Fig. 13). At the cytosolic side, the hydroxylated compounds are mainly conjugated by sulfotransferases, whereas at the luminal side they are conjugated by UGTs. Although the sequential reactions catalyzed by P450s and UGTs are potentially very complicated, they are ultimately determined by kinetic parameters, such as the substrate specificity for each enzyme and the solubility of substrates and their corresponding metabolites.

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B. Functional Interaction of P450s and UGTs in the ER 1. P450R and P450 a. Topology The topology of P450R and P450 and the formation of their complex on the ER membrane are important controlling factors for electron transfer. P450R is a 78‐kDa flavoprotein associated with the cytoplasmic surface of the ER membrane. Two binding models have been proposed (Black and Coon, 1982). The first places the NH2 and COOH termini on opposite sides (Ccyt‐Nlum, type III topology) of the membrane with the hydrophobic segment spanning the lipid bilayer. An alternative model (Ccyt‐Ncyt) proposes both termini to be located on the cytoplasmic side of the membrane. The latter model is supported by the fact that the NH2‐ terminal anchor domain, which is not cleaved as a signal peptide, has hydrophobic characteristics and is acetylated (Haniu et al., 1986). These observations indicate that the NH2‐terminal region of the domain is likely to be located on the cytosolic face (Fig. 13). This mode of binding facilitates more rapid movement across the surface of the ER than that of the type III topology. Furthermore, P450R is solubilized by trypsin treatment, indicating that the catalytic domain does not interact with ER membrane. P450s that do not undergo posttranslational NH2‐terminal modification have an amino‐terminal membrane‐anchoring segment associated with the ER membrane with type III topology. In this case, the NH2‐terminus is found in the lumen and the COOH‐terminus in the cytoplasm (Fig. 13). Furthermore, the hydrophobic tail and surface of the P450 enzyme can interact with the hydrophobic core region of the membrane. The basic residues are located above the hydrophobic region where they can interact favorably with the head group of phospholipids in the polar region of the membrane (Zhao et al., 2006). The corresponding surface was identified in P450 17a (P45021A2) by a combination of chemical modifications and mass spectrometry (Izumi et al., 2003). In this membrane‐binding orientation, the P450 enzyme forms a channel for hydrophobic substrates in the lipid bilayer to access the active site. The channel also opens to the cytosol, providing access for less hydrophobic substrates. A hydrophobic compound might enter the substrate‐binding site from the membrane surface (Zhao et al., 2006). Comparison of the ligand‐free and ligand‐bound structure has identified structurally plastic regions that undergo conformational change in response to ligand binding. The most plastic regions are putative membrane‐ binding motifs involved in substrate access or substrate binding. b. Interaction Between P450R and P450 Interaction between P450 and P450R molecules is required for electron transfer to occur (Hlavica et al., 2003; Lewis and Hlavica, 2000; Peterson et al., 1976; Taniguchi et al., 1979).

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Localization of these two proteins on the two dimensional (2‐D) surface of the ER membrane serves to both concentrate reactants and increase the frequency of their interaction. In general, these processes include at least three elemental steps: (1) formation of an active P450R–P450 complex; (2) electron transfer between these complexes; and (3) dissociation of P450R and P450. The rate of P450 reduction by the first and second electron can be divided into two steps (Fig. 7): Reduction ratefirst electron ¼ Ka kET1 ðP450RÞðP450Þ

ð6Þ

Reduction ratesecond electron ¼ Ka kET2 ðP450R or b5 Þðoxygenated P450Þ ð7Þ where Ka is the association constant between P450 or b5 and reductase at concentrations represented by the terms in parentheses, and kET1 and kET2 are first and second electron transfer rate constants (Archakov and Bachmanova, 1990). The first and second electron is supplied from the P450R, but the second electron is also supplied via the cyt b5 (Eq. 7) Transfer of the second electron is the rate‐limiting step of the overall reaction (Imai et al., 1977). Therefore, the rate of formation of hydroxylated product (ROH) may be determined from Equation 7. However, the reactions on the ER membrane are very complicated. In the Singer‐Nicolson model (1972), it is believed that these proteins are distributed randomly in two dimensions, in which the movement and orientation of reactants are restricted. The ER membrane serves to concentrate the reactants and hence to increase the frequency of their interaction. As already discussed, the detergent‐solubilized reductase has activity toward P450, whereas the protease‐solubilized reductase, which lacks the membrane‐ binding domain, is not functional in the reduction of P450s. These observations suggest that the interaction of the reductase and P450 with the ER membrane is essential for eYcient electron transfer. Both b5R, with an N‐terminal myristoylated anchor, and b5, with a C‐terminal tail‐anchored hydrophobic domain, are associated with the membrane and are exposed to the cytosolic compartment. Tonegawa et al. (2005) proposed that the interaction between b5R and b5 is described by a (2‐D) random walk model. The concentration of P450R in the membranes has been estimated to be 1/10 to 1/40 of total P450s (Estabrook et al., 1971; Watanabe et al., 1993). Therefore, the reductase must interact with all P450s. This raises the important question as to how the reductase can interact specifically with P450s. Two possible mechanisms are conceivable for functional interactions between the P450R and the P450 in microsomal membranes. One model suggests that the interactions are brought about by the lateral motion and subsequent collision of these proteins on the plane of the ER membrane

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(Taniguchi et al., 1979). Alternatively, the proteins may exist in the ER membrane as functional clusters in which the interactions can take place directly (Peterson et al., 1976). In addition to the interaction between P450 and P450R, P450–P450 interactions have also been observed in reconstituted systems (Kelley et al., 2005). The presence of one P450 (P4501A2) enzyme can aVect the function of another P450 (P4502B4). Interestingly, this interaction depends on ionic strength, indicating that P450–P450 complexes are formed by charge–pair interactions. Although electron transfer between two proteins, including the P450R/P450s, P450R/b5, b5/P450s and homo/hetero P450‐P450 systems, have been studied in vitro, the interaction of these proteins on the natural membrane has yet to be fully addressed. Kemper and coworkers (Ozalp et al., 2005; Szczesna‐Skorupa et al., 2003) have used bimolecular fluorescence complementation techniques to study P450 interactions in a natural membrane context within living cells. Interactions of P450s with P450R were detected, as well as homo‐oligomerization of P4502C2, but not P4502E1. The interaction of P4502C2 with P4502E1 is weak, but homo‐oligomerization of P4502C2 is mediated by the signal anchor sequence. In contrast to self‐oligomerization, the catalytic domain can mediate an interaction of P4502C2 with P450R. These data strongly suggest that interaction of reductase with P450 is mainly dependent on electrostatic interactions between the soluble catalytic domains of both enzymes. However, clustering of P450s on the ER membrane was detected. Studies of the rotational mobility of P450s indicate that P450 oligomers may dissociate when the enzyme binds to the reductase (Yamada et al., 1995). The hetero‐oligomerization of adrenal P450scc with P45011b (P45011B1) (Ikushiro et al., 1992) and P4502B4 with P4501A2 (Kelley et al., 2005) modulates the enzyme activity. In addition to P450s, P450R can transfer an electron to cytochrome b5, heme oxygenase and squalene monooxygenase. This raises the important question as to how the P450R interacts specifically with these electron acceptors, including P450. The highly conserved conformational motifs of the P450s may play a role in the molecular recognition process (Mestres, 2005). However, the structure of b5 (Argos and Mathews, 1975) is significantly diVerent from that of P450 (Johnson and Stout, 2005) and heme oxygenase (Lad et al., 2003; Schuller et al., 1999; Sugishima et al., 2002) enzymes. It is well known that the soluble P450R domain, which lacks the N‐terminal membrane‐binding domain, cannot reduce b5, which also lacks the N‐terminal membrane‐binding domain. Nevertheless, eVective electron transfer occurs in detergent‐solubilized enzymes, which retain the membrane‐ binding domain. Furthermore, the soluble domain of the reductase cannot directly reduce the microsomal bound P450s. These observations suggest that hydrophobic interactions between the membrane‐binding domains of both

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enzymes are necessary for eVective electron transfer, whereas the electrostatic interactions between the soluble reductase and heme domain are less important. Thus, the hydrophobic region between the proteins ensures the correct orientation and juxtaposition of the binding sites at the proximal surface of the P450 and the dimethylbenzene ring of the FMN molecule. The functional complex formed between these proteins may only be transient, but movement of the FAD domain aids the orientation process (see Section II). The FMN domain as a flavodoxin‐like carrier can donate an electron to several diVerent electron acceptors. These proposals may explain why numerous P450s and other electron acceptors can be reduced by a single P450R molecule. However, both the protease solubilized b5R and b5, which lack a membrane‐binding domain, can eYciently exchange an electron (Kimura et al., 2003), whereas protease solubilized P450R cannot transfer electrons to protease solubilized b5 (Iyanagi and Mason, 1973). 2. P450 and UGT a. Topology As mentioned earlier, P450s are located on the cytosolic side of the ER, whereas UGTs are thought to be located within the lumen of the ER (Fig. 13). UGTs are synthesized as precursors of about 530 residues, which include a 20‐amino acid signal peptide that mediates integration of the polypeptide chain into the ER (Fig. 8). The signal peptide is cleaved during protein maturation of the enzyme. The UGTs have a single 17‐amino acid transmembrane segment and a 26‐amino acid cytoplasmic tail at the C‐terminal end of the molecule. The catalytic domain of the UGTs is localized on the luminal surface of the ER (Radominska‐Pandya et al., 2005). On the other hand, microsomal aldehyde dehydrogenase, which lacks a signal sequence is a tail‐anchored protein localized to the cytoplasmic face of the ER (Masaki et al., 2003). A 45‐amino acid C‐terminal deletion mutant of UGT1A9, which includes the transmembrane segment, is water‐soluble (Kurkela et al., 2004). However, the activity of this truncated UGT1A9 is significantly reduced suggesting that the membrane‐binding segment is involved in the enzyme activity. A mutation within this region of UGT1A9, Y486D, causes Gilbert’s and CN type II syndromes (Yamamoto et al., 1998). However, UGT1A1 isoform may contain a putative internal membrane‐associated helix (Ciotti et al., 1998). The microsomal UGTs have broad substrate specificity. Based on protein sequence analysis of UGT isoforms, it is generally accepted that the variable N‐terminal domain binds substrate and therefore determines the substrate specificity, whereas the C‐terminal domain binds the common substrate, UDP‐ GlcUA (Meech and Mackenzie, 1997). This analysis indicates that microsomal UGT enzymes consist of two domains. Compared with mammalian Golgi type II

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membrane‐associated UGT proteins (Clum‐Ncyt topology), which have relatively narrow substrate specificity and two tightly associated domains, the domains of microsomal UGT interact more loosely. The structure of plant UGT71G1, which has a GT‐B fold, indicates that the active site is buried in the cleft region between the N‐ and C‐terminal domains (Shao et al., 2005). Furthermore, the two domains move in response to substrate binding. In microsomal UGT, the most variable amino acids are located in the N‐terminal substrate‐binding domain (Iyanagi, 1991). PhotoaYnity labeling experiments have demonstrated that Phe90 and Phe93 in this region are directly involved in the catalytic activity of UGT1A10 isoform (Xiong et al., 2006). It is likely that the active site of UGT is buried in the cleft region between the N‐ and C‐terminal domains. b. Interaction Between P450 and UGT In general, membrane proteins containing a single transmembrane (TM) domain are able to interact at the catalytic and TM domains. However, interactions between P450 and UGT are mainly confined to the TM domains, although the interaction between the short N‐terminal tail of the P450 and catalytic domain of UGT, or the short C‐terminal tail of UGT and catalytic domain of P450 may also occur (Fig. 13). Two diVerent TM helices, TMP450 and TMUGT, in a lipid bilayer can interact to form three diVerent dimers: TMP450‐TMP450, TMP450‐TMUGT, and TMUGT‐TMUGT. The monomer‐dimer equilibrium can be described by the individual equilibrium constants (Merzlyakov et al., 2006). These constants may be determined from the specificity between isoforms of both enzymes, and their respective concentrations within the cell. To avoid the formation of a ternary complex, a P450 must dissociate from P450R before interaction with UGT. In this case, interactions between the TM domains and between catalytic domains must be considered within the homodimer or heterodimer of P450 or UGT. Taura et al. (2000) showed that rat UGTs coeluted with rat P4501A1 using a bovine serum albumin‐conjugated Sepharose 4B column. Fremont et al. (2005) studied the formation of the complex using a coimmunoprecipitation method. The UGT2B7, UGT1A6, UGT1A1, and P4503A4 were immunoprecipitated with specific antibodies for each enzyme. Takeda et al. (2005) reported a coimmunoprecipitation of P4503A4 with UGT2B7. These data suggest that UGT isoforms may form complexes with each other, and UGT isoforms may interact with P450s. Ikushiro et al. (1997) demonstrated evidence for hetero‐oligomers between UGT1A isoforms and UGT2B1. This complex was copurified using specific Sepharose‐conjugated antibodies directed against either UGT1A or UGT2B1 isoforms and confirmed by crosslinking experiments. The eVects of UGT complex formation on the stimulation of glucuronidation of testosterone and uptake of UDP‐glucuronic acid (UDP‐GlcUA) by UDP‐N‐acetylglucosamine

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(UDP‐GlcNAc) have also been examined. Alkaline pH‐induced dissociation of the complex was associated with the loss of UDP‐GlcNAc–dependent stimulation of glucuronidation, suggesting that two functional states of UGTs with diVerent kinetic parameters correspond to the monomer and oligomer form of UGTs in the membrane. The UDP‐GlcNAc–dependent stimulation of UDP‐ GlcUA uptake into the microsomal vesicles was also aVected by the extent of complex formation. These results suggest that complex formation of the UGT isozymes aVects the UDP‐GlcNAc–dependent stimulation of glucuronidation via stimulation of UDP‐GlcUA uptake. Meech and Mackenzie (1997) engineered two forms of UGT2B1 that were catalytically inactive when expressed alone, but catalytically active when coexpressed. They further demonstrated that the N‐terminal domain of UGT participates in dimer formation. The interactions between P450/P450, P450/UGT, and UGT/UGT in the ER membrane may modulate the enzyme activity and substrate specificity. Kelley et al. (2005) reported P450‐P450 interaction using a mixed reconstituted system containing P450R, P4502B4, and P4501A2. The enzyme activity decreased at high ionic strength, indicating disruption of the P450R‐P450 and P450‐P450 complexes. Additionally, they suggested a substrate‐specific electrostatic interaction between P450 enzymes. Takeda et al. (2005) reported that the activity of morphine‐3‐glucuronide formation by UGT2B7 is reduced by addition of purified P4501A2 and P4502C9 in a concentration‐dependent manner. Ishii et al. (2001) reported that morphine‐6‐glucuronide formation is enhanced by the UGT hetero‐oligomer formation, indicating the change of substrate specificity. The protein–protein interaction between P450 and UGT would permit reactions to proceed more eYciently in cells. The rat P4501A1 and UGT1A6 were coexpressed in yeast microsomes (Ikushiro et al., 2004). However, eYcient coupling of hydroxylation and glucuronidation in the sequential metabolism of 7‐ethoxycoumarin was not observed in this combination. The data suggest that either a functional complex between these isoforms is not formed, or that the transfer of substrate from the active site of P450 to UGT is eYciently not coupled with the formation of complex. Another example of the relationship between a UGT oligomer and its function has been reported for UGT1A1. In CN type II patients the interaction between the mutant forms of UGT1A1 and wild‐type enzyme is dominant negative, and the activity toward bilirubin is reduced (Koiwai et al., 1996). Further experimental studies support the homodimerization of recombinant UGT1A1 and may explain this dominant negative eVect (Ghosh et al., 2001). However, it is very diYcult to predict the interaction between enzymes on the ER membrane. A major question concerning the interaction between P450s and UGTs is how these enzymes interact with each other and how this

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interaction modulates their activity. It is likely that contact between the TMs or the catalytic domains may induce a conformational change in the active site of the enzymes.

C. Broad Substrate Specificity In general, enzymes have a high degree of substrate specificity. However, the phase I and phase II DMEs display broad, overlapping substrate specificities. Structural studies suggest that these enzymes have a highly plastic active site, which can accommodate a wide variety of substrates. Interestingly, the DNA repair enzymes, which recognize modified DNA as cytotoxic endobiotics, also have broad substrate specificity. It appears that these enzymes have acquired conformational plasticity, allowing them to recognize and metabolize multiple substrates. This may be a common feature of DMEs. Indeed, as described previously, protein–protein interactions may modify the activity and substrate specificity of the enzyme. 1. Microsomal Enzymes a. P450/UGT The substrate diversity of microsomal P450s suggests an easily accessible active site, whereas the mitochondrial P450s have a relatively narrow substrate specificity. The microsomal P450s can each bind and metabolize a number of substrates of diVerent sizes, shapes, and stereochemistry (Clodfelter et al., 2006; Johnson and Stout, 2005; Yanao et al., 2005). The structures of P450s, including 2C5, 2C9, and 2B4 suggest that the ability of adjusting their binding sites to substrates that diVer in size, shape, and polarity is to be responsible for the broad substrate specificity. After studying the structure of P4502B4, Zhao et al. (2006) proposed a model in which the most plastic regions of the enzyme are membrane‐binding motifs involved in substrate access or substrate binding. The substrate binding site is largely hydrophobic, but polar interactions can contribute to selectivity for substrate binding and to the orientation of substrates. The relatively large active site cavities have the potential to bind two or more drug substrates simultaneously. The Phe120, Asp301, Thr309, and Glu216 have been identified in microsomal P4502D6 substrate binding and catalysis. The Phe120 acts to control the orientation of the aromatic ring of substrates with respect to the heme moiety (Rowland et al., 2006). The Thr309 is expected to be the conserved threonine (Thr) involved in proton delivery to the catalytic water, as proposed in bacterial P450cam (P450101) (Imai et al., 1989; Nagano and Poulos, 2005). In addition to its potential role in molecular oxygen activation, Thr309 may play an important structural role within the active site crevice (Keizers et al., 2005; van Waterschoot et al., 2006).

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The microsomal UGTs display broad, overlapping substrate specificities (King et al., 2000; Radominska‐Pandya et al., 1999; Tukey and Strassburg, 2000), whereas the Golgi‐type UGTs have a relatively narrow substrate specificity (Negishi et al., 2003; Sugahara et al., 2003). Although the structure of microsomal UGT is not known, it is likely that these enzymes contain the GT‐B fold consisting of two domains. Control of conformational flexibility between the two domains is probably controlled in the same way as plant UGT71G1 (Shao et al., 2005). Therefore, UGTs may also have a highly plastic active site due to the relative movement of the two domains, allowing the cavity to accommodate a wide variety of substrates. Because the active site of the P450 faces the ER membrane, the UGT may preferentially accept hydroxylated substrates from the ER membrane (Fig. 13). b. Carboxylesterase (CE) CEs, which are located on the luminal side of the ER, are typical phase I enzymes and play a major role in the metabolism, detoxification and elimination of xenobiotic and endobiotic esters (Imai, 2006; Satoh and Hosokawa, 1998). The enzymes also play a critical role in the activation of prodrugs and can hydrolyze a wide variety of ester, amide, and thioester substrates (Huang et al., 2005b). The structure of rabbit and human enzymes is composed of a catalytic domain, ab domain, and a regulatory domain (Bencharit et al., 2002, 2003). The active site of this family shares a common mechanism of hydrolysis involving a catalytic trial composed of a serine, histidine, and either an aspartic acid or a glutamic acid residue. The enzymes contain a ‘‘small rigid’’ pocket, which recognizes the ester linkage, and a ‘‘large flexible’’ pocket, which recognizes a large region of the substrate. The anticancer prodrug CPT‐11, which is a potent topoisomerase I inhibitor, is hydrolyzed by carboxyesterase (Slatter et al., 1997) and the product, SN38, is conjugated by UGT1A1, UGT1A7, and UGT1A9 (Ando et al., 2000; Ganng et al., 2002; Iyer et al., 1998; Tukey et al., 2002; Villeneeuve et al., 2003). c. Epoxide Hydrolase (EH) The epoxidation reaction of xenobiotics is catalyzed by P450s. The epoxide is then hydrolyzed by EHs to give the corresponding vicinal 1,2 diol (Arand et al., 2003; Gomez et al., 2006). The enzymes exist as microsomal and soluble isoforms. The microsomal EH contains an N‐terminal membrane anchor, whereas soluble EH lacks this anchor. The structure of soluble EH suggests that the catalytic mechanism proceeds through a covalent alkylenzyme ester intermediate with an active site aspartate nucleophile. The hydrolysis of this intermediate requires that an oxygen atom of the enzyme is incorporated into the vicinal diol product. The microsomal EH also shares the same mechanism. Interestingly, the C‐terminal catalytic domain is similar to that of haloalkane dehalogenase from Xanthobacter autotrophicus, which hydrolyzes carbon‐halogen

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bonds via a mechanism involving an aspartate nucleophile and an alkylenzyme ester intermediate. Moreover, both these domains share a a/b hydrolase fold. These findings suggest that the active site of EHs have diverged to accommodate a strikingly broad range of xenobiotic substrates (Argiriadi et al., 1999). 2. Other Related Enzymes a. NAD(P)H:Quinone Oxidoreductase (NQO1, DT‐Diaphorase) NQO1 is a FAD‐containing flavoprotein that catalyzes quinone. Detoxification is transcriptionally induced in response to various agents, including xenobiotics and oxidants (Talalay et al., 1995). This enzyme catalyze the two electron reduction of a broad range of quinones to hydroquinones (Anusevicius et al., 2002; Iyanagi and Yamazaki, 1970; Tedeschi et al., 1995a,b). The structure of the enzyme has suggested a direct hydride transfer from reduced FAD to ˚ above the flavin quinones (Li et al., 1995). The duroquinone ring stacks 5 A ring with carbonyl oxygen atoms running almost parallel throughout the length of the isoalloxazine ring of the FAD cofactor. Steady‐state kinetic and docking studies support a model in which quinones with aromatic rings in the quinone nucleus interact with the active site to optimize ‐ring‐stacking interactions with the isoalloxazine ring. Substrate binding is stabilized by hydrogen‐bonding interactions with His161 in the active site (Zhou et al., 2003). The larger quinones rotate along the quinone carbonyl axis, relative to the duroquinone position (Winski et al., 2001). Thus, the enzyme modifies the shape of the active site to accommodate diVerent substrates. b. Sulfotransferase (SULT) SULTs catalyze the transfer reaction of the sulfate group from the donor 30 ‐phosphoadenosine 50 ‐phosphosulfate (PAPS) to an acceptor group of numerous substrates (Nagata and Yamazoe, 2000). The cytosolic SULTs transfer sulfate to small molecules, such as steroids, bioamines, and xenobiotics, whereas their counterparts in the Golgi membrane catalyze the transfer of sulfate to large molecules, such as glycosaminoglycans and proteins. Although the cytosolic‐ and Golgi‐associated SULTs share a similar PAPS‐binding site and catalytic core, the substrate‐binding site is diVerent (Negishi et al., 2001). The binding site of membrane SULTs is a large open cleft with a hydrophilic surface, whereas a deep hydrophobic pocket provides the substrate‐binding site in the cytosolic SULTs. The complementary structure of the substrate with the hydrophobic surface of the binding pocket appears to determine the substrate specificity. c. DNA Repair Enzyme DNA damage caused by xenobiotic and endobiotic alkylation reagents creates lesions that are both mutagenic and cytotoxic (Mishina et al., 2006; O’Brien, 2006). Although the DNA repair enzymes

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are not DMEs, they can recognize modified DNA as a toxic endobiotic. Interestingly, the structure of the oxidative DNA/RNA repair enzyme AlkB suggests that the substrate‐binding ‘‘lid’’ has a flexible conformation, which may enable docking of diverse alkylated nucleotide substrates in an optimal catalytic geometry (Yu et al., 2006). Thus, AlkB appears to have developed an elegant molecular design in which these flexible protein segments recognize invariant nucleic acid backbone features to facilitate high‐aYnity docking of chemically diverse bases into a conserved catalytic core. The oxidative dealkylation is catalyzed by a dioxygen activation reaction involving a high‐valent iron(IV)‐oxo intermediate species that can function as an oxidant (Yu et al., 2006), as discussed in Section II.

D. Biotransformation of Phenol Compounds Aromatic hydrocarbons including benzene, benzo(a)pyrene and estrogens, are metabolized by phase I enzymes to give many metabolites. These metabolites, such as phenols, arene oxides, quinones, dihydrodiols, and diol epoxides, are conjugated by phase II enzymes to glucuronides, sulfate, and glutathione derivatives, which are water‐soluble, detoxified products. The phenol derivatives are formed by P450 mediated hydroxylation or by the hydrolysis of epoxides. These compounds are converted to quinone derivatives by autoxidation or peroxidases, and their carbonyl groups may be enzymatically reduced to a hydroxyl moiety (Fig. 14). However, quinone compounds, including anticancer drugs, undergo one‐electron reduction by flavoenzymes resulting in a semiquinone radical. The reaction of molecular oxygen with semiquinone radical generates an active oxygen species. In addition, the arylating quinones react with cellular nucleophiles such as thiols on cysteine residues of proteins, glutathione, and detoxifying agents such as N‐acetyl cysteine (Fig. 14). 1. Hydroxylation of Aromatic Compounds and Their Biotransformation Benzene, which is a highly toxic compound, is hydroxylated to phenol by P4502E1 and then converted to p‐benzoquinone by autoxidation or peroxidases (Ross, 2005). In contrast, its epoxide is converted to diol by EH and oxidized to o‐quinone. Glutathione (GSH) reacts directly with benzoquinone, whereas the hydroquinone is mainly conjugated by UGTs (King et al., 2000) or SULTs (Shangari et al., 2005), and it is readily excreted in bile or urine. Benzo(a)pyrene is activated by P450s. P4501A1/1A2 and P4501B1 are responsible for the metabolic activation of this compound to epoxide

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FIG. 14 The one (1e )‐ and two (2e )‐electron oxidation‐reduction reactions of quinone (Q) and active intermediates. RH and SOD indicate aromatic compound and superoxide dismutase, respectively.

intermediates, which are converted, with the aid of EH, to the powerful carcinogen, 7,8‐diol‐9,10‐epoxide (Conney, 1982; Fujii‐Kuriyama and Mimura, 2005; Miller, 1978; Shimada and Fujii‐Kuriyama, 2004). The diol derivatives of benzo(a)pyrene are oxidized to o‐quinone via semiquinone by autoxidation or peroxidases. However, aldo‐keto reductase (AKR) catalyzes the formation of quinone derivatives by two‐electron reduction. Fang et al. (2002) suggest that several UGTs may play an important role in the overall glucuronidation of benzo(a)pyrene‐trans‐7,8‐dihydrodiol, which is a precursor of the carcinogen derivatives. UGT1A1, 1A7, A8, 1A10, and potentially 1A8 play an important role in the glucuronidation of these compounds. Estrogens are metabolized by oxidative and conjugative reactions (Samunio et al., 2003). They are good substrates of P4501A1/1A2 and 1B1 that generate predominantly 2‐ and 4‐hydroxy‐catecholestrogen derivatives (2OHCE and 4OHCE), respectively. Both CEs are detoxified by several enzymatic processes, such as glucuronidation, sulfation, and methylation. UGT1A8, UGT1A9, and UGT2B7 are primarily involved in the inactivation of 4OHCEs (Thibaudeau et al., 2006). UGT1A1, UGT1A3, UGT1A8, and UGT1A9 are also involved in the inactivation in 2OHCEs. The dihydrodiols are oxidized to o‐quinones by autoxidation or peroxidases. In addition to conjugation reactions, the quinone derivatives, which are derived from benzene, benzo(a)pyrene, and estrogens, react directly with the proteins and DNA (Bolton et al., 2000; Zahid et al., 2006).

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2. One‐ and Two‐Electron Oxidation and Reduction of Quinones The flavoenzymes can reduce quinones (Qs) in one‐electron, two‐electron and mixed‐type reduction (Anuservicius et al., 2002; Cenas et al., 2004; Iyanagi and Yamazaki, 1970; Matsuda et al., 2000). Yamazaki (1971) proposed a tentative definition of the one‐electron and two‐electron transfer mechanism. Figure 15 illustrates the electron transfer between reduced flavin enzyme (E‐FlH2) and Q. When the reaction proceeds along route a, it is termed a two‐electron mechanism regardless of the lifetime of the one‐ electron transfer intermediate (E‐FlH ‐QH ). Thus, a one‐electron mechanism implies that the intermediate (E‐FlH ‐QH ) releases only semiquinone radical (QH /Q ) via a reaction path indicated by route b. Anusevicius et al. (2005) proposed that the mechanism of quinone reduction by flavoenzymes may be determined by the stability of the intermediate, E‐FlH ‐QH . NQO1 catalyzes a typical two‐electron transfer reaction, involving direct hydride transfer from FAD to quinones. In addition to NQO1, the short‐chain dehydrogenase (SDR) and aldo‐keto reductase (AKR), which do not contain the prosthetic group, catalyze the two‐electron reduction of carbonyl compounds (Matsunaga et al., 2006). These enzymes, which involve direct hydride transfer also mediate two‐electron transfer reactions. In contrast, P450R, NADH:ubiquinone oxidoreductase (complex I), ferredoxin‐NADPþ reductase and NOSs are typical one‐electron transfer enzymes (Cenas et al., 2004; Fu et al., 2004; Iyanagi and Yamazaki, 1969, 1970; Matsuda et al., 2000). In P450R and NOS reductase domains, the fully reduced states (V and IX in Fig. 5) of FMN are the most active species with quinones (Yamamoto et al., 2005). The rate of quinone reductions, including antitumor adriamycin and mitomycin C are stimulated by CaM (Fu et al., 2004; Matsuda et al., 2000). However, hydroquinone compounds are oxidized in the one‐electron reaction by peroxidases or autoxidation (Ohnishi et al., 1969; Sawada et al., 1975). The one‐electron reduction of quinones or one‐electron oxidation of hydroquinone results in the formation of semiquinone radicals, in which their cytotoxicity may depend on the reactivity with molecular oxygen (Cenas et al., 2004). The superoxide radical is formed from the direct reaction of oxygen with the semiquinone radical. Although this active oxygen radical dismutates to

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FIG. 15 The mechanism of electron transfer in the overall bivalent oxidation‐reduction. E‐FlH2 indicates enzyme‐bound reduced flavin, and E‐FlH ‐QH corresponds to the principal formed one‐electron transfer intermediate.

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hydrogen peroxide and oxygen, the reaction is also catalyzed by superoxide dismutase (SOD). The superoxide radical reacts with nitric oxide (NO), resulting in the formation of peroxynitrite (ONOO ) (Fig. 14). The peroxide also reacts with ferrous iron (Fenton reaction), resulting in a hydroxyl radical (HO ) and high‐valent iron (IV)‐oxo intermediates (FeO2þ or Fe4þ ¼ O) (Groves, 2006; Yamazaki and Piette, 1990, 1991). The eYciency of hydroxyl radical formation depends on the nature of the iron chelator. The high‐valent iron (IV)‐oxo intermediates may be generated in the presence of a ligand such as ADP. As discussed in the activation of oxygen by P450 (see Section II.B.4.c), this active intermediate is also formed by one‐electron reduction of ferrous oxygen complex. The P450R can eYciently donate electrons to ligand‐bound Fe2þO2. The HO and Fe4þ ¼ O intermediates may also be involved in the complex formed from iron and anthracyclines (Zweier et al., 1986) or bleomycins (Burger et al., 1981, 1983). The hydroxy radical (HO ) and high‐valent iron intermediate (Fe4þ ¼ O) can extract a hydrogen atom from the substrate (as discussed in Section II. B.4.c). Therefore, these may be a major cause of quinone‐mediated toxicity in the presence of iron (Fe2þ), causing damage to lipids, proteins, and DNA (West and Marnett, 2006). For example, anthracyclines, which have quinone moieties in their structure, are potent antineoplastic drugs that cause apoptosis of breast cancer cells (Ravi et al., 2005). The flavoenzymes catalyze one‐electron reduction of anthracyclines (Bachur et al., 1979; Fu et al., 2004; Matsuda and Iyanagi, 1999; Powis, 1987; Vasquez‐Vivar et al., 1997). However, these compounds are glucuronized by UGT2B7, and their metabolites subsequently inactivated (Innocenti et al., 2001). All quinones are redox cycling agents that generate reactive oxygen (Fig. 14). In addition, the arylating quinones react with cellular nucleophiles such as thiols on cysteine residues of proteins, glutathione, and detoxifying agents such as N‐acetyl cysteine, forming covalently linked quinone‐thiol Michael adducts that retain the ability to function in redox cycling (Cadenas, 1989; Ollinger et al., 1989). Wang et al. (2006) proposed that Michael adduct formation between arylating quinone and cysteine residues on secretory proteins can disrupt the formation of correct disulfide bonding, causing protein misfolding, inducing ER stress, and ultimately leading to cell toxicity. In addition to xenobiotic compounds, physiological compounds are also important substrates in these pathways. For example, dopamine is oxidized to dopamine quinone, generating reactive oxygen radicals during the one‐ electron reduction (Paris et al., 2005). The neurotoxicity of dopamine quinone is caused by the formation of a complex with iron. The NQO1 mediated two‐electron reduction of aminochrome, which is derived from dopamine may reduce the toxicity (Segura‐Aguilar and Lind, 1989). In addition to these events, dopamine quinone binds covalently to a variety of proteins via reduced cysteine residues (LaVoie et al., 2005).

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V. Concluding Remarks It is interesting to consider the coordinate structure/function of the phase I and phase II DMEs in the ER membrane (Fig. 13). The P450s and UGTs display broad overlapping substrate specificities, which together constitute a general enzyme system within the organism. The DMEs including P450 and UGT have a highly plastic active site, which can accommodate a wide variety of substrates. Furthermore, P450R can donate electrons to 50 microsomal P450s. The microsomal electron transport systems facilitate the biotransformation and detoxification of xenobiotics with drastically diVerent chemical structures. In addition, sequential biotransformation by both the P450R/ P450 system and UGTs constitute one of the major routes for drug metabolism. These reactions play a vital role in the metabolism and detoxification of xenobiotic (exogenous) and endobiotic (endogenous) compounds. The plant P450R/P450 system has a similar cellular organization to the mammalian system, although the GTs are soluble enzymes. The localization and functions of these enzymes strongly suggest that the DMEs are evolutionarily related to secondary metabolism of small molecules in plants. In addition, both the P450 and UGT are thought to acquire the diversity during the coevolution by ‘‘animal‐plant warfare’’ (Holton et al., 1993; Lewis, 2001; Lewis et al., 1998). The P450 genes are distributed on several chromosomes, although they are often found in clusters, but P450R is encoded by only one gene (Fig. 4). In contrast, UGTs are encoded by complex (UGT1A family) and cluster (UGT2 family) genes (Fig. 10A). UGT1 gene complex is unique, and not observed for other drug‐metabolizing activities, including phase I, II, and III enzymes. This unique gene complex has not been found in plant and fish. A similar gene complex, which encodes the protocadherin proteins is expressed in distinct patterns in the nervous system. The gene organization of the UGT1 and protocadherin genes resembles that of the immunoglobulin and T‐cell receptor gene clusters, with the tandemly arrayed variable region (V) exons followed by a diverse set of constant (C) exons (Fig. 10B). However, the diversity of the UGT1A and protocadherin proteins is due to alternative pre‐mRNA splicing between diVerent ‘‘variable’’ exons and ‘‘constant’’ exons. Furthermore, the phase I and II enzymes may have evolved synergistically for the metabolism of druglike molecules. The metabolic pathways for the hydrophobic compounds found in mammalian cells appear to necessitate compartmentalization in the hydrophobic ER membrane (Fig. 13). Finally, the P450R/P450 system and UGTs are now recognized as the principal enzymes involved in the detoxification of xenobiotics in the ER membrane.

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Acknowledgments The author thanks Dr. Jung‐Ja Kim, Department of Biochemistry, Medical College of Wisconsin, USA, and Dr. Peter Mackenzie, Department of Clinical Pharmacology, Flinders University School of Medicine, Flinders Medical Center, Bedford Park, Australia, and Drs. Yoshitsugu Shiro, Shingo Nagano, Hiroshi Sugimoto, Akihiro Kikuchi, and Atsuko Kohara of Biometal Science Laboratory, RIKEN Harima Institute/SPring 8 for useful discussions and suggestions.

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Further Reading Backes, W. L., and Kelley, R. W. (2003). Organization of multiple cytochrome P450s with NADPH‐cytochrome P450 reductase in membranes. Pharmacol. Ther. 98, 221–233. Bock, K. W., and Kohle, C. (2004). Coordinate regulation of drug metabolism by xenobiotic nuclear receptors: UGTs acting together with CYPs and glucuronide transporters. Drug Metab. Rev. 36, 595–615. Bukowski, M. R., Koehntop, K. D., Stubna, A., Bominaar, E. L., Halfen, J. A., Munck, E., Nam, W., and Que, L., Jr., (2005). A thiolate‐ligated nonheme oxoiron (IV) complex relevant to cytochrome P450. Science 310, 1000–1002. Caspersen, C. S., Reznik, B., Weldy, P. L., Abildskov, K. M., Stark, R. I., and Garland, M. (2007). Molecular cloning of the baboon UDP‐glucuronosyltransferase 1A gene family: Evolution of the primate UGT1 locus and relevance for models of human drug metabolism. Pharmacogenet. Genomics 17, 11–24. Csala, M., Banhegyi, G., and Benedetti, A. (2006). Endoplasmic reticulum: A metabolic compartment. FEBS Lett. 580, 2160–2165. Guillemette, C. (2003). Pharmacogenomics of human UDP‐glucuronosyltransferase enzymes. Pharmacogenomics J. 3, 136–158. Gutierrez, A., Grunau, A., Paine, M., Munro, A. W., Wolf, C. R., Roberts, G. C., and Scrutton, N. S. (2003). Electron transfer in human cytochrome P450 reductase. Biochem. Soc. Trans. 31, 497–501. Iyanagi, T., Emi, Y., and Ikushiro, S. (1998). Biochemical and molecular aspects of genetic disorders of bilirubin metabolism. Biochim Biophys Acta 1407, 173–184. Massey, V. (2000). The chemical and biological versatility of riboflavin. Biochem. Soc. Trans. 28, 283–296. Tasic, B., Nabholz, C. E., Baldwin, K. K., Kim, Y., Rueckert, E. H., Ribich, S. A., Cramer, P., Wu, Q., Axel, R., and Maniatis, T. (2002). Promoter choice determines splice site selection in protocadherin alpha and gamma pre‐mRNA splicing. Mol. Cell. 10, 21–33. Wolkoff, A. W. (2005). The hyperbilirubinemias. In ‘‘Harison’s Principles of Internal Medicine’’ (D. L. Kasper, E. B. Braunwald, A. S. Fauci, S. L. Hauser, D. L. Longo, and J. L. Jameson, Eds.), 16th ed., pp. 1817–1821. McGraw Hill, New York. Yueh, M. F., Bonzo, J. A., and Tukey, R. H. (2005). The role of Ah receptor in induction of human UDP‐glucuronosyltransferase 1A1. Meth. Enzymol. 400, 75–91.

Effects of Growth Factors on Testicular Morphogenesis Sarah Mackay and Robert A. Smith Division of Neuroscience and Biomedical Systems, Institute of Biomedical and Life Sciences, University of Glasgow, Glasgow, UK G12 8QQ

Since the discovery of the sex‐determining gene Sry in 1990, research effort has focused on the events downstream of its expression. A range of different experimental approaches including gene expression, knocking‐out and knocking‐in genes of interest, and cell and tissue culture techniques have been applied, highlighting the importance of growth factors at all stages of testicular morphogenesis. Migration of primordial germ cells and the mesonephric precursors of peritubular myoid cells and endothelial cells to the gonad is under growth factor control. Proliferation of both germ cells and somatic cells within the gonadal primordium is also controlled by cytokines as is the interaction of Sertoli cells (with each other and with the extracellular matrix) to form testicular cords. Several growth factors/growth factor families (e.g., platelet‐derived growth factor, fibroblast growth factor family, TGFb family, and neurotrophins) have emerged as key players, exerting an influence at different time points and steps in organogenesis. Although most evidence has emerged in the mouse, comparative studies are important in elucidating the variety, potential, and evolution of control mechanisms. KEY WORDS: Testis development, Sex differentiation, Growth factors, Morphogenesis, AMH, FGF9, PDGF, Neurotrophic factors. ß 2007 Elsevier Inc.

I. Introduction In 1986 developmental biologist Rita Levi‐Montalcini and biochemist Stanley Cohen were awarded the Nobel Prize for Physiology or Medicine for their discovery of nerve growth factor in the 1950s (see Levi‐Montalcini, 1998). International Review of Cytology, Vol. 260 Copyright 2007, Elsevier Inc. All rights reserved.

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It had taken over 3 decades for their work to be fully appreciated; moreover, the fundamental importance of growth factors in the control of proliferation and diVerentiation in both normal and abnormal development is still being elucidated. Morphogenesis of the testis provides a useful representative model system in which to study growth factor control of cell biological events as it involves, at various stages, cell migration, proliferation, diVerentiation, apoptosis, epithelial–mesenchymal interactions, cell–matrix interactions, and vasculogenesis (Brennan and Capel, 2004; Mackay, 2000; Ross and Capel, 2005). Growth factors have been implicated in the control of similar phenomena in other organ systems (Chen et al., 2004; Lu et al., 2006; Michael and Davies, 2004; Serls et al., 2005; Shimogori et al., 2004; Thisse and Thisse, 2005; Tickle, 2003; White et al., 2006). Over the last 15 to 20 years a considerable amount of research eVort has been directed to investigate the role of growth factors at specific stages and on specific cell types during testis development (Abo‐Elmaksoud and Sinowatz, 2005; Mackay, 2000). Both in vivo and in vitro approaches have been used (Cupp et al., 2000; Ricci et al., 2004). The application of genetic approaches, both knocking‐in and knocking‐out genes of interest, has also resulted in a wealth of new information (Behringer et al., 1990; Brennan and Capel, 2004; Xia et al., 2004). The elucidation of the role of growth factors in testicular morphogenesis is key to understanding disorders of testicular function in adulthood, which may have their origins in the developmental period. For example, ‘‘testicular dysgenesis syndrome’’ in humans is a collection of common disorders (germ‐ cell cancer, cryptorchidism, hypospadias, and low sperm counts) thought to have a common origin during the developmental period related to abnormal functioning of Sertoli and Leydig cells (Sharpe et al., 2003).

II. Comparative Testicular Morphogenesis A considerable amount of research data on testicular morphogenesis has been accumulated using the mouse and the rat as experimental animals; these laboratory rodents are assumed to be representative mammals, although mouse development diVers in several ways from that found in most mammals (Mu¨ller, 1997). Important developmental mechanisms tend to be conserved, but it is nonetheless desirable to widen the scope of observation and experimentation to a larger number of species to gain an insight into mammalian morphogenesis. Moreover, occasionally a species will come to light with a remarkable mode of development, which elucidates the potential of basic mechanisms.

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Female moles belonging to several species of the genus Talpa are unique in having bilateral ovotestes (Barrionuevo et al., 2004), with a smaller ovarian portion bearing normal follicles and a larger testicular part that lacks germ cells, but has abundant Leydig cells producing testosterone and spherical testicular cords composed of immature Sertoli cells surrounded by peritubular myoid cells. In contrast to other mammals, the first signs of sex diVerentiation appear in females rather than in males, with the appearance of the medulla and cortex in females before testis diVerentiation is seen in males. The authors speculate that the first role of the sex‐determining gene, SRY, in male moles may be to avoid this regionalization. A further diVerence between moles and other mammals is that entry of female germ cells to meiosis is delayed with respect to testis diVerentiation and occurs after birth. Timing of entry to meiosis is known to be delayed in species where there are more well‐defined ovarian cords which produce steroidal hormones during the delay period (Byskov, 1979). Importantly, this work shows key events of testicular diVerentiation (e.g., mesenchymal cell migration, medullary cord formation, development of the vascular system, and the tunica albuginea) can occur in the absence of SRY. Furthermore, given that the medullary cord cells lack morphological features of Sertoli cells and do not express their product, anti‐Mu¨llerian hormone (AMH), these elements of testicular diVerentiation can develop in female moles in the absence of typical pre‐ Sertoli or Sertoli cells. Follicular granulosa cells are known to have the potential to transform into Sertoli cells after oocyte loss (Taketo‐Hosotani et al., 1985), which might explain the development of testicular features in the medullary region of female moles where PGCs are largely absent (Barrionuevo et al., 2004). Insights into the evolution of the molecular genetics of vertebrate sex determination have been provided by studies on the chicken (Smith and Sinclair, 2004). Sex in birds is determined by a ZZ/ZW system rather than an XX/XY system and female is the heterogametic sex. Furthermore, only the left gonad becomes an ovary while the right regresses. The SRY gene is absent in birds, but several other genes important for mammalian sex determination are also expressed in the chicken, though with diVerent expression patterns. These include the orphan nuclear receptor steroidogenic factor‐1 (SF‐1), the Wilm’s Tumor‐associated protein WT‐1, and the LIM homeobox protein LHX; SF‐1 and WT‐1 activate SRY expression in mammals and presumably activate other sex determinants in the chicken (Smith and Sinclair, 2004). SF‐1 and WT‐1 also cooperate with SOX9 to turn on expression of AMH in mammals, but in the chicken AMH expression precedes that of SOX9. These genes are not sex‐linked in the chicken, but there are candidate sex‐determining genes in birds and other organisms which are sex‐ linked: Drosophila Doublesex and Caenorhabditis (C.) elegans Mab‐3– related transcription factor 1 (DMRT1) (Z‐linked) and avian, sex‐specific,

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W‐linked (ASW) and female‐expressed transcript 1 (FET1), which are both W‐linked. A further diVerence in birds is the importance of estrogens; evolutionary pressure in mammals, where there is a highly developed placenta and intrauterine development, has led to the establishment of other mechanisms so that testis diVerentiation can proceed in the presence of maternal sex steroids (Wolf, 1999). In the chicken, expression of the estrogen receptor is seen in both sexes prior to sex diVerentiation, but is later downregulated in males as well as in the right female gonad (Smith and Sinclair, 2004). As in mammals, diVerentiation and proliferation of Sertoli cells within cords is a key step in testis diVerentiation, but there does not appear to be a prominent coelomic blood vessel (Smith and Sinclair, 2004), as seen at the time of cord formation in mouse testis diVerentiation (McLaren, 1983). The migration of mesonephric cells into the developing mouse testis is necessary for cord formation (Buehr et al., 1993a; Martineau et al., 1997; Tilmann and Capel, 1999). Incoming cells contribute to the endothelial (Martineau et al., 1997), peritubular myoid cell (Nishino et al., 2001), and Leydig cell populations (Merchant‐Larios and Moreno‐Mendoza, 1998). Mesonephric cell migration cannot be induced into XX mouse gonads after E12.5 unless the XX gonads are depleted of germ cells, which are by this stage meiotic and would otherwise antagonize mesonephric cell migration (Yao et al., 2003). Investigation of the control of this process has shown that although mesonephric migration into XX gonads may be induced by addition of recombinant AMH in culture, no abnormalities are seen in AMH‐deficient male mice (Ross et al., 2003). It is also known that signaling by the receptor for platelet‐derived growth factor (see Section III.B.1) acts on migrating mesonephric cells indirectly (Brennan et al., 2003). In an elegant study using chicken–quail cocultures, no migration of QCPNþ quail mesonephric cells was seen in cocultured male chicken gonads in the presence of the PDGFR inhibitor AG1296 (tyrphostin), though extensive immigration of QCPNþ cells occurred in controls (Smith et al., 2005). Mouse cells migrated in chicken–mouse interspecific cocultures in the absence of Sry in the chicken; in the presence of inhibitor mesonephric cell migration was reduced. Results that PDGFR‐a is expressed in the gonads rather than in the mesonephroi suggest the PDGF signaling necessary for mesonephric cell migration may be indirect. A component of the phosphatidylinositol 3‐kinase pathway involved in PDGF signaling, the kinase P13KC2a is expressed in the chicken testis at the time of sex diVerentiation and concomitant with mesonephric cell migration. It remains to be seen whether this kinase is expressed at the time of mammalian gonadal development. In conclusion, Sry induces mouse mesonephric cell migration indirectly, via a conserved pathway shared with birds in which PDGFR signaling is implicated. There is no obvious eVect on general cord formation when mesonephric cell migration is inhibited in the avian system, implying that promotion of cord

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organization may not be the primary function of this migration in all vertebrates (Smith et al., 2005). Temperature‐dependent sex determination is shown in many reptiles including all crocodilians, many turtles, and several lizards (Crews, 2003; Ferguson and Joanen, 1983; Western and Sinclair, 2001). Despite this major diVerence between reptiles and mammals, genetic mechanisms controlling gonadal morphological diVerentiation appear to be conserved: as in the mouse, AMH expression marks Sertoli cell diVerentiation in the alligator testis (Western and Sinclair, 2001). In the mouse, upregulation of AMH expression is controlled by SOX9, but in alligator and chicken gonads this AMH upregulation occurs before that of SOX9 indicating a diVerent control mechanism must operate (Western and Sinclair, 2001). Thus, although a similar repertoire of genes may be involved in gonadal diVerentiation during both genetic and environmental sex determination, a diversity of control mechanisms may operate (Yao and Capel, 2005). Marsupial mammals are also of interest; for example, the tammar wallaby has been reported as showing extensive sexual dimorphisms preceding any morphological diVerentiation of the gonads (O et al., 1988). This finding is at odds with the classical view of mammalian sexual diVerentiation that after the testis‐determining gene triggers testis diVerentiation, androgen from Leydig cells promotes male reproductive tract development while AMH from Sertoli cells inhibits female tract development. Although such exceptions to the rule are illuminating they may be very rare; evidence from another marsupial, Monodelphus domestica, suggests androgens play a role in development of the scrotum (Russell et al., 2003). Furthermore, a study by Coveney et al. (2002) shows that treatment of tammar wallaby pouch young with estradiol benzoate from the day of birth results in profound eVects on genital ducts and smaller scrota than those of controls; these eVects appear to result from alteration of normal testicular production of both AMH and androgens as well as from direct eVects of estrogen on target tissues indicating that androgens may play a role in this species. A further puzzle in marsupials is the question of a mesonephric contribution to the testis. As mentioned previously, in the mouse mesonephric cells contribute peritubular myoid cells, which are important in contributing fibronectin to the basal laminae of developing testicular cords, stabilizing their structure (Buehr et al., 1993a; Capel et al., 1999; Martineau et al., 1997; Merchant‐Larios et al., 1993). In M. domestica the mesonephros is still acting as the functional kidney at the time of birth and so presumably cannot contribute cells during testicular diVerentiation around the time of birth (Mackay et al., 2004a; Xie et al., 1996). Testis cords will develop in sea turtle gonads cultured without adjacent mesonephroi (Moreno‐Mendoza et al., 2001) and no evidence for a mesonephric contribution to the testis of the red‐eared slider turtle has been found (Yao and Capel, 2005).

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A common denominator between the eVects of sex‐determining genes and environmental factors has been identified: control of metabolic rate (Kraak and de Looze, 1993; Mittwoch, 2004). Testis‐determining genes may act by increasing metabolic rates rather than by directly determining Sertoli cell diVerentiation. Mittwoch proposes that the testis‐determining genes SRY and SOX9 bring about an increase in metabolic rate in tissues in which they are active, increasing cell proliferation and other developmental processes such as migration; similar eVects are produced by a temperature rise in ectothermic vertebrates (Mittwoch, 2004).

III. Cell Migration A. Germ Cells In the male mammal there are four periods of germ cell movement, whether active or passive. The first occurs when the primordial germ cells (PGCs) migrate from the hindgut wall to the genital ridge. The second is when the germ cells relocate from the lumen of the testicular cord to the basement membrane in postnatal life. Thirdly, preleptotene and leptotene spermatocytes must translocate from the basal to the adlumenal compartment of the seminiferous tubule for further development in adult life (Lui et al., 2003a). Lastly, the active motility of spermatozoa is important in fertilization. Growth factors are likely to be involved in control at all stages. An elegant study was performed in which mice expressing green fluorescent protein (GFP) in early germ line cells were used to investigate migratory activity of PGCs (Molyneaux et al., 2001). Slices of embryo at diVerent stages of development were cultured and time‐lapse recordings made, over periods from 8 to 10 h, using confocal microscopy. Observations showed active motility in PGCs from E9.0 to E12.5 occurring within four phases of behavior: (1) (E9–E9.5), PGCs are highly motile while they are within the gut wall; (2) (E9–E9.5), before the mesentery forms, they emerge rapidly from the gut; (3) (E10–E10.5) PGCs migrate into the genital ridges from the dorsal body wall; and (4) (E11.5) PGC movement slows; in females the PGCs move randomly, whereas in males most traced cells move in the medial‐posterior direction (Molyneaux et al., 2001). The authors suggest the long‐held view that PGCs migrate up the dorsal mesentery is a misconception, because in these experiments the majority of PGCs had migrated from the gut into the dorsal body wall before the mesentery had formed. Explanted E8.5 migratory PGCs will move preferentially toward E10.5 genital ridges in culture (Godin et al., 1990); this chemotropic eVect is

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mediated by TGFb1 or a closely related molecule, as it can be abolished by anti‐TGFb1 antibody (Godin and Wylie, 1991). The c‐kit/stem cell factor signaling pathway (see Section V.A) is required for normal migration (McLaren, 2003). In mice homozygous for a mutation in the W gene (which encodes the c‐kit ligand for stem cell factor; see Section V.A) migration of PGCs lags behind wild‐type and heterozygotes with a larger proportion of germ cells remaining in the gut wall (Buehr et al., 1993b). Donovan and coworkers (1986) proposed that once PGCs reach the gonad anlage in the mouse they undergo major phenotypic changes resulting in a loss of motile capability. We have shown however, that in the female at least the potential for migration is not lost by oocytes because germ cells are shed from cultured mouse ovarian explants peaking at day 7 postnatally (Mackay et al., 1992). This appears not to be just a mechanism for elimination of dying germ cells, as seen in humans to reduce the pool of oocytes (Motta and Makabe, 1986), because the germ cells in our study retained good cytoplasmic integrity (as evidenced by TEM) and SEM examination confirmed the presence of regular lamellipodia and filopodia. Oocytes displaying migratory phenotypes were also reported in a separate study of neonatal mice by Wordinger et al. (1990) with germ cells released at the surface from healthy nonarteritic primordial follicles indicative of retention of motility. Stromal cell‐derived factor 1 (SDF1) is a member of the CXC family of chemokines (i.e., cytokines which may activate or attract leucocytes). The normal migration of PGCs in zebrafish depends on the interaction between SDF1 and its G‐protein–coupled receptor CXCR4 (Knaut et al., 2003). This interaction is also required in the mouse, where the receptor is detected at E9.5 on migratory germ cells and its ligand in the entire dorsal body wall, with higher staining in the neural tube floorplate, the mesonephros, and adjacent mesenchyme (Molyneaux et al., 2003). Migration of germ cells in vitro can be perturbed by adding high local concentrations of SDF1. In embryos with a targeted mutation for the receptor, germ cells do not colonize the genital ridges correctly, although PGCs do colonize the hindgut. In these mutant embryos a progressive reduction of germ cells occurs during and after colonization of the genital ridges. When tissue slices from E10.5 embryos were cultured in the presence or absence of SDF1, PGC numbers in SDF1‐treated slices showed a statistically significant increase compared with controls, indicating that SDF1 acts as a growth or survival factor for PGCs in the mouse (Molyneaux et al., 2003). A role for FGF signaling in mouse germ cell migration has been shown (Takeuchi et al., 2005). Evidence includes analysis by RT‐PCR of cDNA which shows E10.5 germ cells express the FGF receptors Fgfr1‐IIIc and Fgfr2‐IIIb (see Section V.5) and results of gain‐of‐function experiments showing FGF2 (a ligand for FGFR1‐IIIc) aVects motility, whereas loss of

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function causes inhibition of cell shape changes in migrating germ cells. Directionality of germ cell movement does not appear to be aVected by FGFs (Takeuchi et al., 2005). Expression of TGFb3 has been found in adult rat germ cells in a stage‐ specific manner extending from the basal to the luminal compartment, being predominant in stages V–VIII of the cycle and diminished at stages IX and X (Lui et al., 2003a,b). Evidence in the adult rat suggests that blood–testis barrier dynamics in vivo are regulated by TGFb2 and TGFb3 (Wong et al., 2004). TGFb3 plays a crucial role in the regulation of Sertoli cell tight junctions via the MEKK2/p38MAP kinase pathway (Lui et al., 2003b), to open the blood–testis barrier to allow migration of preleptotene and leptotene spermatocytes.

B. Peritubular Myoid Cells/Endothelial Cells/ Mesonephric Cells Migration of cells from the mesonephros to the gonad is a male‐specific event (Martineau et al., 1997). Migrating cells include peritubular myoid cells (PMCs) and other interstitial cells (Buehr et al., 1993a; Nishino et al., 2001) in addition to endothelial cells necessary for angiogenesis in the developing testis (Brennan et al., 2002; Jeays‐Ward et al., 2003). 1. Platelet‐Derived Growth Factor Platelet‐derived growth factor (PDGF) stimulates mitosis in cells of mesenchymal origin (Heldin and Westermark, 1990), it is involved in mesenchymal–epithelial interactions (Uzumcu et al., 2002a), and it belongs to the PDGF‐vascular endothelial growth factor family. Several biologically active PDGF molecules are known; four are homodimers (PDGF‐AA, PDGF‐BB, PDGF‐CC, and PDGF‐DD) and there is also a heterodimer, PDGF‐AB (Mariani et al., 2002). In a study of PDGF‐AA and PDGF‐BB and their receptors (PDGFRs), Gnessi and coworkers (1995) used a battery of techniques including immunohistochemistry, Northern blot analysis, and RNA isolation to elucidate the expression of these molecules in rats at various developmental stages from the late fetal stage, in vivo and in vitro. Expression of PDGF A‐chain, B‐chain, and PDGFR (both a and b subunits) was found from the earliest stage examined; expression rose postnatally, remaining high for the first 5 days of postnatal life and then declined to lower levels in 15‐day animals, and had virtually disappeared in older animals. During prenatal and early postnatal stages expression of PDGFs was seen in Sertoli cells (PDGFs) and of PDGFRs in PMCs, whereas in adult animals expression of PDGFs and PDGFRs was only seen in Leydig cells. Postnatal production of PDGFs was

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found to be controlled in a dose‐dependent fashion by follicle‐stimulating hormone (FSH) (Gnessi et al., 1995). These authors were also able to show a chemotactic eVect of all PDGF isoforms and of Sertoli cell‐conditioned medium on isolated peritubular myoid cells, which was inhibited by anti‐PDGF antibodies. Brennan et al. (2003) carried out coculture experiments to investigate the eVect of PDGF on recruitment of mesonephric cells in developing mouse gonads. In control experiments, although XY gonads recruited mesonephric cells, XX gonads did not. However, if 50 ng/ml of PDGF‐AA, ‐BB, or ‐AB was added to the culture medium, cells were recruited into the XX gonad from GFP‐expressing mesonephroi after 48 h in vitro; all migrating GFP cells were PECAM‐positive endothelial cells. To investigate the possibility that mesonephric cell migration was abnormal in Pdgfr‐a / XY gonads, cultures were established using diVerent combinations of Pdgfr‐a / mesonephroi or Pdgfr‐a / gonads and wild‐type/Pdgfr‐aþ/ XY mesonephroi or gonads (mesonephroi were GFP‐positive). Two days later cultured gonads were examined for the presence of GFP‐positive cells. Results showed Pdgfr‐a expression is not required on mesonephric cells for migration; however, migration was severely impaired if the gonad was Pdgfr‐a / and the mesonephros was Pdgfr‐aþ/ . The authors interpreted this data to mean that PDGFR‐a signaling acts on migrating mesonephric cells indirectly, activating a second signal in gonadal cells, which then promotes migration (Brennan et al., 2003). In the same year, similar experiments were carried out to investigate the expression and function of PDGF‐BB and its receptor, PDGFR‐b, during mouse testis morphogenesis (Puglianiello et al., 2003). Immunoreactivity for PDGFR‐b was found in the mesonephros, but not in the gonad at E11.5. However, at E12.5 and E13.5 PDGFR‐b–expressing cells progressively appeared within the interstitial tissue of the male gonadal ridge. An earlier study by this group had shown mesenchymal cells migrating to the testis from the mesonephros are characterized by their expression of the p75 neurotrophin receptor (see Section III.B.4) and can be isolated by immunomagnetic sorting with anti‐p75NTR antibody from total mesonephric cell suspensions (Campagnolo et al., 2001). Virtually all of these selected cells were found to also express the PDGFb receptor. At E12.5 and E13.5 Northern blot analysis showed PDGF‐BB mRNA in gonads, with a higher content in males; in situ hybridization also showed a higher expression of PDGF‐BB mRNA in the testis, mainly in the interstitial population. Exposure to PDGF‐BB stimulated both mitosis (as indicated by a 2.5‐fold increase in [3H]‐TdR incorporation) and migration of mesonephric mesenchymal cells, inducing shape changes associated with chemotaxis such as rearrangement of actin filaments and the development of edge ruZes. Although migration occurred at low PDGF‐BB concentrations, higher concentrations were required for the

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mitogenic eVect. The authors suggest a gonadally released gradient might induce migration of mesonephric mesenchymal cells, which would then be exposed to higher levels once in the gonad, triggering proliferation. The possible signal transduction pathways involved in the PDGF‐BB–induced stimulation of mitosis and migration were also investigated. Both mitogen‐ activated protein kinases (MAPK) and phosphatidylinositol‐3 kinase (PI3K) pathways were found to be required, as both the MAPK inhibitor U0126 and the PI3K inhibitor Ly294002 were shown to inhibit migration and proliferation in assays in vitro (Puglianiello et al., 2003). Synthesis of PDGF‐BB in the mouse testis was demonstrated by immunolocalization by Ricci et al. (2004): PDGF‐BB was present at a low level in the male genital ridge at E11.5 and the interstitial compartment of the testis was weakly positive at E13.5. At E11.5 receptor immunolocalization was restricted to the coelomic epithelium and mesonephric mesenchyme, but not the gonad in the case of PDGFR‐b. In the case of PDGFR‐a, low level immunostaining was seen in some cells of the coelomic epithelium and at the boundary between the gonad and mesonephros and to a lesser extent in the mesonephric mesenchyme. By E13.5 the coelomic epithelium over the genital ridge was more positively stained for PDGFR‐b as were the interstitial and peritubular cells, although staining for the a receptor chain was less evident. The role of PDGF‐BB as a migratory factor for male mesonephric cells was investigated using Boyden’s migration chambers to carry out an in vitro migration assay. Dissociated mesonephric cells were seeded in the upper side of the chambers whereas lower chambers were filled with medium alone or supplemented with 100‐ng/ml PDGF‐BB, which was found to strongly increase migratory activity as compared with controls. Conditioned medium (CM) from E13.5 testicular cell cultures also strongly increased migratory activity; this eVect of CM was inhibited by the addition of an anti‐PDGF‐BB neutralizing antibody (Ricci et al., 2004). An organ culture approach was used to investigate the role of the PI3K signaling pathway in testis diVerentiation. A high dose of the PI3K inhibitor Ly294002 totally inhibited cord formation in E11.5 male urogenital ridges cultured for 4 days in vitro (div) and also inhibited testicular cell reaggregation in a dose‐dependent manner. 2. Hepatocyte Growth Factor Hepatocyte growth factor (HGF), originally identified acting as a mitogenic factor for hepatocytes (Nakamura et al., 1984), is a powerful angiogenic factor stimulating endothelial cell motility and growth (Bussolino et al., 1992). HGF and its receptor c‐met have been implicated in regulating the detachment and emigration of myogenic precursor cells in the dermomyotome (Birchmeier and Gherardi, 1998). Mesonephric cells isolated from E13.5 mouse embryos showed significantly increased ( p ¼ < 0.001) migratory

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activity when cultured in the upper side of Boyden chambers whose lower chambers were filled with medium supplemented with HGF (100–400 U/ml), compared with cells cultured with medium alone (Ricci et al., 2002). 3. Transforming Growth Factor b Superfamily As well as the transforming growth factor (TGF)b family, this superfamily includes the activin/inhibin family, AMH and members of the bone morphogenetic protein (BMP) family (Lui et al., 2003a) apart from BMP‐1, which is a metalloproteinase (Kessler et al., 1996). In mammals there are three homodimer isoforms of TGFb: TGFb1, TGFb2, and TGFb3 (Josso and di Clemente, 1999). a. Transforming Growth Factor b3 In an immunohistochemical study on the expression and action of the three TGFb isoforms during rat testis development, higher concentrations of TGFb3 were found during embryonic development from E16 to the time of birth, with significantly lower concentrations postnatally. Although TGFb1 was expressed in Sertoli cells, gonocytes and some interstitial cells during embryonic testis development, and TGFb2 staining was specific for Sertoli cells at E14, TGFb3 expression at this time was restricted to cells in the border region between the testis and mesonephros. Intensely staining cells appeared to be preperitubular, around testicular cords, although isolated interstitial cells were also positive. The authors speculate preperitubular cells may express TGFb3 to induce migration or diVerentiation; further investigation should be directed to clarifying this potential role (Cupp et al., 1999). b. Anti‐Mu¨llerian Hormone Synthesized by, and released from pre‐Sertoli cells (Josso, 1994), AMH, also known as Mu¨llerian inhibiting substance (MIS), functions to induce Mu¨llerian duct regression in the male. Additional roles for AMH include regulation of germ cell maturation and gonadogenesis, control of testicular descent, inhibition of lung maturation, and suppression of tumor growth (Lee and Donahoe, 1993). For many years there has been speculation about a possible role in testis development, because AMH produces the ‘‘freemartin’’ condition in nature, in which female bovine embryos can be masculinized if linked to a male twin by placental anastomoses, allowing the passage of AMH to the female (Jost et al., 1972). Organ culture experiments have been carried out to determine whether AMH is involved in the control of mesonephric cell migration, specifically, whether AMH could induce migration of mesonephric cells into an XX mouse gonad (Ross et al., 2003). Mouse gonads were detached from urogenital complexes of E11.5 and E12.5 embryos and cultured recombined with mesonephroi from ROSA 26 embryos which express a lacZ reporter gene. After 24 h

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extensive mesonephric cell migration occurred into the E11.5 XY gonad but not the XX gonad. However, if the culture medium contained 15‐mg/ml recombinant human AMH numerous cells did migrate into the female gonads, albeit in reduced numbers compared with the males. Migration could not be induced in the case of ovaries extracted at E12.5, suggesting a restricted time window during which diVerentiation may be influenced by AMH (Ross et al., 2003). A further finding was that in E11.5 XX gonads cultured with AMH a coelomic blood vessel and coelomic epithelial thickening was seen as in normal XY gonads; these features are not normally seen in XX gonads, where follistatin acts downstream of Wnt4 to block mesonephric cell migration (see Section IV.B). No testis abnormality is seen in AMH null mutants. Therefore, if AMH does have a role in normal testis morphogenesis, its loss must be compensated by another factor or factors. AMH exerts its eVects by activating a BMP‐like signaling pathway involving the phosphorylation of downstream Smad1 protein (Clarke et al., 2001; Goue´dard et al., 2000; Visser et al., 2001; Xavier and Allard, 2003). Signaling by TGFb family cytokines is mediated through a complex of two serine/ threonine kinase receptors (type I and type II) which then activate two cytoplasmic receptors, receptor‐regulated Smads (R‐Smad) and common Smad (Smad4). Type II is the primary receptor which binds the ligand, phosphorylating the type I receptor which then phosphorylates R‐Smad, which in turn interacts with Smad4 (di Clemente et al., 2003). The type I receptor for AMH is likely to be a BMP‐specific type‐I receptor: ALK‐2 (also known as ActR‐IA), ALK‐3 (also known as BMPR‐IA), and/or ALK‐6 (also known as BMPR‐IB); which is responsible for mediating the action of AMH and may vary under diVerent conditions or in diVerent cell types (Shimasaki et al., 2004). Smad proteins are related to the protein product of the Drosophila gene Mothers against decapentaplegic (Mad) (GraV et al., 1996). Mad‐related proteins have been found in a variety of organisms and act as intracellular transducers of the TGFb family. AMH induces the phosphorylation of the BMP‐specific R‐Smad, Smad1, and its association with Smad4; the complex moves to the nucleus (di Clemente et al., 2003) where it presumably attaches to a Smad‐ binding element on the promoter of target genes (Massague´ and Chen, 2000). In addition to the Smad pathway, AMH can also function via other signaling pathways such as b catenin/LEF‐1, as in the case of Mu¨llerian duct regression (Allard et al., 2000) or NFkB in inhibition of breast cancer cell growth (Segev et al., 2000). To determine whether other members of the TGFb family, which use the same Smad eVector proteins as AMH, could substitute for it, XX gonads were cultured with beads coated with recombinant BMP2 or BMP4 protein (Ross et al., 2003). Growth of vasculature was induced, but because neither gene is expressed in normal development, a diVerent BMP may be involved in the regulation of mesonephric migration (Ross et al., 2003).

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4. Neurotrophic Factors The neurotrophin family includes nerve growth factor (NGF), brain‐derived neurotrophic factor (BDNF), neurotrophin (NT)‐3, and NT‐4/5 (Bothwell, 1995). All are able to bind to the low aYnity receptor P75/NTR, but also have their own high‐aYnity receptors: trkA for NGF, trkC for NT3, and trkB for NT4/5 and BDNF (Barbacid, 1995; Cupp et al., 2002). Cells that migrate from the mesonephros to the mouse gonad are characterized by the presence of the low‐aYnity NGF receptor (NGFR), p75 NT receptor (p75NTR) on their surface (Campagnolo et al., 2001). A cluster of p75/NTR‐positive cells can be identified in the mesonephros at E10.5 and in a region adjacent to the gonad from E11.25 (15–16 tail somites) where they spread into the gonad from E11.5, filling the testicular stroma by E12.5. Cells positive for p75/NTR can be isolated from the gonad by immunomagnetic selection; if cultured for up to 3 div on Matrigel nearly all cells express the peritubular myoid cell marker (Tung and Fritz, 1990), a‐smooth muscle actin after 2 div (Campagnolo et al., 2001). The specific ligand and its source remains to be identified for the mouse. No NT can be detected in the early mouse gonad until E14.5 when NT‐3 is expressed by testicular mesenchymal cells (Russo et al., 1999). It may be that NTs are active in the developing mouse gonad at concentrations below the limit at which we can currently measure their presence. In the rat, a clearer story has emerged: immunohistochemistry shows migratory mesenchymal cell expression of high aYnity trkC receptors, whereas embryonic Sertoli cells express NT3 (Cupp et al., 2000; Levine et al., 2000a). When signaling of NT3 through its trkC receptor is inhibited by a tyrphostin inhibitor (AG879), testicular cord formation is inhibited in E13 testis organ cultures and few to no cells migrate from labeled mesonephroi to testes. Furthermore, a reduction in SOX‐9 gene expression is seen in the diVerentiating testis (Cupp et al., 2003). These findings show the importance of NT3 as a chemotactic signal attracting mesonephric cells necessary for the establishment of testicular cords. The human fetal testis (at 14–19 weeks’ gestation) shows expression of mRNA for NGF, NT3, NT4, BDNF, high‐aYnity receptors trkA, trkB, trkC, and low‐aYnity receptor p75. Expression of NT4 mRNA and protein and p75 is localized to the peritubular cells (Robinson et al., 2003).

IV. Vascular Development A diVerentiating mouse testis can first be identified on E12–E12.5 by its striped appearance, due to newly formed testicular cords and blood vessels in between (Fig. 1). Especially obvious is the peripheral vessel just below the coelomic

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FIG. 1 Micrographs of E13.5 A male and B female urogenital complexes. TC, testicular cord, arrow indicates coelomic vessel; O, ovary; M, mesonephros.

surface, referred to by some authors as the coelomic vessel (Brennan et al., 2002). The association in time between testicular cord formation and a new pattern of vasculature in the male has led authors to speculate on a possible role for vascular formation in testicular organogenesis (Brennan et al., 2002; Martineau et al., 1997; Merchant‐Larios et al., 1993). Incoming cells from the mesonephros discussed earlier (see Section III.B) include contributors to the endothelial population (Buehr et al., 1993a; Martineau et al., 1997; Merchant‐ Larios et al., 1993). In fact, a large proportion of the male vasculature

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(including the coelomic vessel) forms from cells that have migrated in from the mesonephros (Brennan et al., 2002).

A. Vascular Endothelial Growth Factor Despite the absence of mesonephric immigration, vascular growth occurs in the XX gonad at the same time as in the XY gonad. This does not appear to stem from assembly of new vessels from large numbers of vasculogenic precursors already present in the ovary or from increased endothelial cell proliferation (Brennan et al., 2002). Expression of the endothelial‐specific growth factor vascular endothelial growth factor (VEGF) shows similar levels of expression throughout the interstitial tissue of both XX and XY gonads, suggesting VEGF is involved in primary vascular growth in both sexes (Brennan et al., 2002). These authors postulated that migration of endothelial cells into the XY gonad may function to increase complexity of the vasculature, perhaps to cater for rapid growth of the testis or to provide for export of testosterone. In fact, their studies with expression of the molecule Ephrin B2, which is expressed specifically in developing arteries, showed that the coelomic vessel is an artery.

B. Follistatin and Bmp2 The Wnt‐4 gene encodes a signaling protein important in the female for suppression of Leydig cell diVerentiation, maintenance of postmeiotic oocyte development, and Mu¨llerian duct development (Vainio et al., 1999). In a study of Wnt4 / mutant mice, the male pattern coelomic vessel was found to form by migration of endothelial cells from the mesonephros as in the male (Jeays‐Ward et al., 2003), indicating a function of Wnt4 in blocking this migration in wild‐type females. Two genes expressed downstream of Wnt4 may be involved: the gene encoding the activin antagonist follistatin (Fst) and that encoding the bone morphogenetic protein Bmp2. In the XX gonad, both Wnt4 and Fst are expressed in somatic cells several layers below the surface coelomic epithelium, whereas Bmp2 is expressed in cells just below the coelomic epithelium. Neither Fst nor Bmp2 are expressed in Wnt4 / XX gonads between E12.5 and E14.5 (Yao et al., 2004). Furthermore, in Fst / XX mutants a coelomic vessel is seen at E12.5 as in Wnt4 / mutants (unfortunately Bmp2 / mutants do not survive long enough to allow investigation of whether a coelomic vessel is present). These results show that although endothelial cell migration and formation of the coelomic vessel is normally XY‐specific, it requires neither Sry expression nor Sertoli cell diVerentiation (Yao et al., 2004). Although the coelomic vessel forms in

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both Wnt4 / and Fst / XX mutants, the branches that run from it between testicular cords in the XY gonad are not seen; this aspect of vascular development, which may play a part in testicular cord morphogenesis, must be separately controlled. A further finding of this study is that germ cells are lost by apoptosis from the ovarian cortex (as well as in the medullary region where it is normal) at E16.5 in Fst / XX mutants as in Wnt4 / mutants (Vainio et al., 1999). The authors suggest that the coelomic vessel could introduce new signals into the cortex which antagonize germ cell survival.

V. Proliferation A. Germ Cells In the past it has proved impossible to maintain isolated PGCs in vitro in the absence of somatic cell feeder layers (De Felici, 2000). However, a cocktail of growth factors and other compounds has been discovered which will allow the survival and proliferation of PGCs in the absence of feeder layers (Farini et al., 2005). This mixture includes stem cell factor/kit ligand, leukemia inhibitory factor (LIF), FGF‐2, BMP‐4, and SDF‐1 together with N‐acetyl‐L‐cysteine, forskolin and retinoic acid.

1. Transforming Growth Factor b Although the main eVect of TGFb is cell cycle arrest, TGFb can either stimulate or inhibit proliferation of diVerent cell types (Josso and di Clemente, 1999). Mouse E8.5 PGCs will increase in number during 5 div when cultured in serum‐free medium conditioned by E10.5 genital ridges, but this increase in proliferation is inhibited in a dose‐dependent manner when TGFb1 is added to the medium (Godin and Wylie, 1991). Isoforms TGFb1, TGFb2, and TGFb3 are all present in the developing rat testis during fetal and neonatal life (Cupp et al., 1999; Gautier et al., 1994; Olaso et al., 1997; Teerds and Dorrington, 1993). In a study in the rat, QRT‐ PCR was used to measure TGFb expression in whole testes taken from rats ranging in age from E15 to PN30. Though the amount of mRNA for TGFb1 was low at E15, it increased at E16, birth, and prepuberty before decreasing after puberty and into adulthood. Expression for TGFb2 was raised at E15 then decreased through E16 and E18; there was a slight elevation from PN0 to PN4 but again expression decreased during pubertal and adult stages. TGFb3 showed higher concentrations from E16 to PN0 and significantly lower concentrations in subsequent stages. The timing of expression of

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TGFb1 and TGFb2 is consistent with a role in regulation of the mitotic arrest which occurs in gonocytes around E17–E18 (Cupp et al., 1999). When E13.5 rat testes were cultured for 2 div with or without TGFb1 and TGFb2, a concentration‐dependent negative eVect of TGFb1 was exerted on the number of gonocytes (Olaso et al., 1998). At 10 ng/ml the maximum reduction was reached; at this concentration TGFb2 had the same eVect as TGFb1. TGFbs had no eVect on BrdU incorporation index in either gonocytes or Sertoli cells. However, when the rate of apoptosis was measured by DNA fragmentation, using the terminal deoxynucleotidyl transferase‐ mediated dUTP nick end labeling (TUNEL) method, a statistically significant increase in the number of TUNEL positive gonocytes was apparent. There was no TGFb1‐induced reduction in the number of gonocytes in testes explanted on E17.5 (when germ cells were quiescent) but after mitosis had been resumed, on PN3, again a reduction was seen. Immunolocalization of type I and type II TGFb receptors showed both receptors present in gonocytes from E13.5 through PN3 and in Leydig cells from E16.5 onward. TGFbs may directly increase apoptosis in gonocytes without aVecting their mitotic activity (Olaso et al., 1998). 2. Activin Another member of the TGFb superfamily, activin, is likely to control the coordinated development of germ cells and Sertoli cells at the onset of spermatogenesis. Gonocyte numbers are significantly increased in testis fragments from PN3 rats cultured with activin and a combination of FSH and follistatin increase the proportion of spermatogonia in the germ cell population after 3 div (Meehan et al., 2000). In situ hybridization and immunohistochemistry on normal rat testis shows gonocytes (but not spermatogonia) express activin bA subunit mRNA and protein. Follistatin mRNA and protein is first expressed at PN3, when gonocytes transform to spermatogonia. Germ cells may therefore regulate their own maturation by production of endogenous activin A and follistatin, aided by Sertoli cells which produce the activin/inhibin bA subunit, the inhibin a subunit, and follistatin. 3. Stem Cell Factor For many years it was known that two mutations in the mouse, for the White spotting and Steel genes decreased germ cell numbers (McCoshen and McCallion, 1975; McLaren, 1994; Mintz and Russell, 1957), but only comparatively recently was the reason for this discovered. The White spotting gene is now known to encode the c‐kit tyrosine kinase receptor (Chabot et al., 1988; Geissler et al., 1988) and Steel encodes its ligand (Copeland et al., 1990; Zsebo et al., 1990), stem cell factor (SCF), which is also known as steel factor

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and mast cell growth factor. The c‐kit gene is expressed in PGCs (Orr‐ Urteger et al., 1990) and the SCF gene along their migratory route and in the genital ridge (Matsui et al., 1990). In vitro, SCF has been shown to be essential for survival (Dolci et al., 1991) and/or proliferation of mouse PGCs (Godin et al., 1991; Matsui et al., 1991). It is possible that in White spotting and Steel mutants PGCs die by apoptosis (Pesce et al., 1993). Proliferating PGCs die in vitro in the absence of somatic cell support, showing features characteristic of apoptosis, such as apoptotic bodies and high levels of tissue transglutaminase, an enzyme activated in apoptosis. Addition of SCF or LIF to cultures significantly reduced the amount of apoptosis after 4–5 h in culture although this eVect was lost after longer times in culture (Pesce et al., 1993). 4. Leukemia Inhibitory Factor There is a direct stimulatory eVect of LIF on PGC proliferation in vitro (Cheng et al., 1994; Dolci et al., 1993; Matsui et al., 1991) and this growth factor will also aid survival of mouse PGCs cultured on feeder layers of the Sertoli cell line, TM4 (De Felici and Dolci, 1991). The low‐aYnity LIF receptor (LIFR) is present on the surface of PGCs and anti‐LIFR antiserum abolishes PGC survival in culture (Cheng et al., 1994). 5. Fibroblast Growth Factor Family This family of heparin‐binding polypeptides is composed of over 23 members (Nie et al., 2006). Although SCF and LIF were found to support survival of PGCs and to allow their proliferation in vitro, rates of growth were only a fraction of those achieved in vivo. Three growth factors were found to be required for long‐term culture of PGCs: SCF, LIF, and basic fibroblast growth factor (Matsui et al., 1992; Resnick et al., 1992), also known as fibroblast growth factor 2 (FGF2). Large multilayered clumps of cells resembling embryonic stem cells can be produced; these cells can form teratomas and contribute to chimeras (Matsui et al., 1992). In a coculture system maintaining Sertoli cells and gonocytes from newborn or PN3 rats, addition of FGF2 from a concentration of 1 ng/ml significantly increased the number of gonocytes after 6 div, acting both as a survival and mitogenic factor (Van Dissel‐Emiliani et al., 1996). Localization of fibroblast growth factors and expression of their receptors has been investigated in vivo in the developing rat testis (Cancilla and Risbridger, 1998; Cancilla et al., 2000). FGF receptors are encoded by four genes (FGFR1, FGFR2, FGFR3, and FGFR4). Each has an intracellular split tyrosine kinase domain and an extracellular domain with up to three immunoglobulin‐like domains. Functional variants IIIb and IIIc arise by

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alternative mRNA splicing of loop III (Cancilla et al., 2000; Han et al., 1993). Additional low‐aYnity receptors, heparin sulphate proteoglycans, are on the cell surface and form a complex with the high‐aYnity receptor for biological activity (Johnston et al., 1995). Expression of FGF1, FGF3, and FGF4, shown by immunohistochemistry, displays discrete cell‐ and stage‐specific localization in the rat testis, which changes over development. Investigation of receptor expression by RT‐PCR shows mRNAs for FGFR1 IIIb and IIIc (in whole testis and isolated Leydig cells), FGFR2 IIIc, FGFR3 IIIc, and FGFR4 in the fetal (E19.5), immature (PN20), and adult (PN90–P100) rat testis (Cancilla et al., 2000). Immunoreactivity for FGF1 and FGF4 is present in fetal gonocytes and Leydig cells, whereas FGF3 immunostaining is not seen in the fetal or immature testis. Immunohistochemistry also shows FGFR2 IIIc in spermatocytes and spermatids of immature and adult testes and in Leydig cells. FGFR3 IIIb is not expressed, so the FGFR3 localized to fetal gonocytes, immature spermatocytes, and specific adult spermatocytes must be due to FGFR3 IIIc (Cancilla and Risbridger, 1998; Cancilla et al., 2000). FGF3 is only found in adult testis and probably acts on elongating spermatids as does FGF4 in an autocrine fashion. The latter may also have an autocrine action on pachytene spermatocytes. Though FGF8 mRNA expression has been found at all stages examined, FGF8 protein may not be present in suYcient amounts to be immunolocalized, as it cannot be detected from E19.5 onward (Cancilla et al., 2000). In the mouse, FGF9, which plays a key role in Sertoli cell proliferation (see Section V.B.1) and diVerentiation (see Section VI.B.1), also acts independently to promote germ cell survival in XY but not XX gonads. Homozygous null mutant XY mice for FGF9 show a significant reduction in gonocyte numbers by E12.5 compared with controls and E11.5 XX null mutants. Further, XY FGF9 / gonads show greater numbers of dying germ cells than XY controls at E11.5, E12, and E12.5. They also fail to develop along the male pathway, subsequently expressing follistatin and Bmp2 (markers of ovarian diVerentiation) and by E14.5 their germ cells enter meiosis as in the ovary (DiNapoli et al., 2006). 6. Platelet‐Derived Growth Factor Rat testicular germ cells undergo two phases of proliferation: in the embryonic period and later at the time when they migrate from the center to the periphery of the seminiferous cord and diVerentiate into type A spermatogonia in early postnatal life (McGuiness and Orth, 1992). PDGF causes the proliferation of germ cells isolated from newborn and early postnatal rat testes in a dose‐dependent fashion in vitro (Li et al., 1997). A mitogenic eVect

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was also demonstrated in this study for 17b‐estradiol, produced by Sertoli cells at high levels during the early postnatal period. However, the eVects of PDGF and estradiol were not additive. 7. Neurotrophic Factors Knockout mice for the high‐aYnity receptors trkA and trkC die at or shortly after birth. Heterozygotes can be mated to produce homozygote trkA knockout mice that survive to PN19; these homozygotes null mutants show a 10‐fold increase in germ cell apoptosis compared with germ cells in wild‐ type mice, although there are no diVerences in germ cell apoptosis during embryonic testis development (Cupp et al., 2002). Testis germ cell numbers in trkA / and trkC / mice have been compared with those of wild‐type mice at E13, E14, E17, and E19. When compared with wild‐type testes, there are more germ cells in trkA / at E13 and E17, although numbers are lower than those in wild‐type testes at E14 and E19. Germ cell numbers in trkC / mice are increased compared to wild‐type mice at E17 but dramatically reduced at E19. These diVerences may result from changes in the expression pattern of genes controlling proliferation, apoptosis, or maturation of germ cells (Cupp et al., 2002). Experiments with human fetal testis explants cultured with the trk‐specific kinase inhibitor K252a show a reduction in gonocyte and peritubular myoid cell number, but little eVect on Sertoli cells (Robinson et al., 2003), indicating a possible role for neurotropic factors in regulation of the proliferation and survival of germ cells and peritubular cells. Glial cell line‐derived neurotrophic factor (GDNF) is part of a family related to TGF‐b now known also to include neurturin, persephin and artemin (Massague´, 1996). Both GDNF and neurturin are expressed in the developing mouse urogenital system (Golden et al., 1999). Mice heterozygous for one GDNF null allele show a depletion of germ cell reserves (Meng et al., 2000) although the gonads of GDNF / mice develop normally (Pichel et al., 1996; Sa´nchez et al., 1996) apart from one report of reversal in the orientation of the ovary in relation to abdominal viscera (Moore et al., 1996). When a human GDNF gene is transfected to mouse Sertoli cells a dramatic amplification of germinal stem cells is seen (Meng et al., 2000) and GDNF has been shown to enhance self‐renewal and increase survival rates of bovine spermatogonial stem cells in culture (Aponte et al., 2006). B. Somatic Cells A sex diVerence in gonadal size can be seen in E13.5 rat embryos, before histological diVerentiation has occurred (Mittwoch et al., 1969). Similarly, after the onset of Sry expression in the mouse between E10.5 and E10.8

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(Bullejos and Koopman, 2001; Hacker et al., 1995) the male gonad doubles its size relative to the female within an 8‐h time window (Schmahl and Capel, 2003; Schmahl et al., 2000). This proliferation is critical to testis formation; when proliferation was blocked between 8 PM on E10 and 4 AM on E11, many XY gonads in each litter failed to develop testicular cords (Schmahl and Capel, 2003). Inhibition of proliferation before or after this critical period produces smaller gonads but does not block testis formation. The male‐specific increased proliferation occurs in at least two stages. Sertoli cells are produced by proliferation in SF‐1 positive cells within the coelomic epithelium before the 18 tail somite stage, approximately equivalent to E11.5 (Karl and Capel, 1998; Schmahl et al., 2000). Identification of cells produced during the second stage of proliferation (19–25 ts) has proved diYcult, as they are not labeled with available markers, though many were labeled with the endothelial marker PECAM (Schmahl et al., 2000). Thyroid hormone plays an important role in controlling Sertoli cell number and the cyclin‐dependent kinase inhibitors p27 Kip1 and p21Cip1 (which regulate progression through the G1 checkpoint of the cell cycle) act as mediators of T3 eVects on Sertoli cell proliferation (Holsberger and Cooke, 2005). 1. Fibroblast Growth Factor Family Fibroblast growth factor 9 (FGF9) has been shown to be crucial to cord formation (Colvin et al., 2001) and without it the gonad diVerentiates along the female pathway (see Section VI.B.1). In situ hybridization has shown a lack of expression of Fgf9 in the developing gonad and mesonephros of E10.5 gonads of both sexes. However, by E11.5 and E12.5 FGF9 is expressed in the XY gonad; by E12.5 it is expressed within testicular cords, whereas the region deep to the coelomic epithelium lacks expression (Colvin et al., 2001). In our laboratory an in vitro approach has been applied to determine the eVect of FGF9 on isolated developing (E14.5) Sertoli cells in culture (Willerton et al., 2004). Addition of FGF9 at a concentration of 10‐ng/ml medium induces enhanced proliferation with an approximately twofold increase in cell number after 7 div. Significantly more cells were labeled with proliferating cell nuclear antigen (PCNA) in cultures treated with FGF9 compared with controls cultured in medium alone. Immunocytochemistry for the FGF9 receptor, FGFr3, showed its localization predominantly in the nucleus of cultured cells, with some cytoplasmic staining in both experimental and control cultures. In vivo, a temporal pattern of expression is seen with immunostaining in the E14.5 testicular cords (both Sertoli and germ cells) but is absent from interstitial tissue, mesonephros, and metanephros. By puberty, FGFr3 immunostaining is localized in spermatogonia and Sertoli cells closest to the tubule basement membrane whereas in the adult, in

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which Sertoli cells do not divide, receptor expression is only seen in spermatogonia (Willerton et al., 2004). In a study of FGF9 function in mouse testis at the time of sex determination (E10.5–E12.5), FGF9 transcripts were detected in XX and XY gonads and mesonephroi at E11.5 by both RT‐PCR and in situ hybridization. Immunocytochemistry showed widespread expression of FGFR1, FGFR2, FGFR3, and FGFR4 in most somatic cells at E11.5 in both sexes. However, FGFR2 expression showed a sexually dimorphic pattern in that it showed nuclear localization only in XY gonads by E11, at the same time as the appearance of SOX9. Not only is SOX9 a marker of Sertoli cell diVerentiation, but its nuclear expression is the first sign of sex diVerentiation after Sry expression in the mouse (Schmahl et al., 2004), so this puts FGFR2 nuclear expression at a key point in the early diVerentiation of Sertoli cells and male sex determination. The nuclear expression of FGFR3 and FGFR2 found by Schmahl and coworkers and in our laboratory may seem anomalous at first. Traditionally the role of the receptor has been seen to transduce the signal (ligand binding) at the cell membrane into a cytosolic one, with subsequent communication involving nuclear translocation of signaling molecules such as kinases. However, there are additional mechanisms whereby ligands may be internalized with or without complexed receptors or signaling components and may translocate to the nucleus to modulate gene expression (Jans and Hassan, 1998). A number of ligands including FGF2 can associate with chromatin; nuclear ligands could alter chromatin structure and gene expression. Indeed, the induction of mitogenesis by FGF1a and FGF1b appears to be dependent on nuclear localization (Jans and Hassan, 1998). Immunofluorescence shows nuclear FGFr3 localization in cultured human breast epithelial cell lines (Johnston et al., 1995) comparable to that shown in our study (Willerton et al., 2004). FGFR3 may have a role in the nuclear function of FGF, a role in transporting it to the nucleus or in storage of FGF in an inactive form in the nucleus, or it may be more actively involved in mediating growth factor function (Johnston et al., 1995). FGF9 may play a part in the development of the chick gonad; there is an FGF9 expression domain in the chick mesonephros adjacent to the gonadal primordium, where FGFR3 is strongly expressed. At the time of gonadal diVerentiation FGF9 expression decreases in the mesonephros, but appears in epithelial cells of gonads of both sexes. Misexpression of FGF9 stimulates cell proliferation and gonadal expansion, whereas inhibition of FGFR3 causes a reduction in gonadal size (Yoshioka et al., 2005). In the perinatal rat, FGF2 is probably a survival factor for Sertoli cells. FGF2 at 1 ng/ml administered to E20, PN0, and PN3 Sertoli cells in coculture with gonocytes increases their number, but not their labeling index after 3 or 6 div (Van Dissel‐Emiliani et al., 1996). FGF2 from germ cells in the

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adult rat can regulate Sertoli cell function, for example, in the secretion of transferrin (Han et al., 1993). FGF4 from elongating spermatids may have paracrine interactions with Sertoli cells expressing FGFR4 (Cancilla and Risbridger, 1998; Cancilla et al., 2000). 2. Platelet‐Derived Growth Factor PDGF is a major mitogen for mesenchymal and connective tissue cells (Gnessi et al., 1997; Heldin and Westermark, 1999). Mesonephric mesenchymal cells immunomagnetically sorted by the presence of the p75 neurotrophin receptor from E12.5 male mouse embryos were shown to respond to PDGF‐BB at concentrations of 50 and 100 ng/ml with a 2.5‐fold increase in [3H]‐TdR incorporation (Puglianiello et al., 2003). Rat PMCs isolated at PN17 and treated with 1.6 nmol PDGF‐AA, PDGF‐ BB, or PDGF‐AB showed an increase in proliferation compared to controls (based on direct cell counts) with a rank order of potencies of PDGF‐BB > PDGF‐AB > PDGF‐AA (Gnessi et al., 1993). However, in a later study, cells isolated slightly later, from PN18 to PN20 rats, failed to show a proliferative response to PDGF‐BB at the same dose when assessed by both direct cell counts and [3H] thymidine incorporation (Chiarenza et al., 2000). Rather than hyperplasia, PMCs in this study appeared to undergo initial contraction, followed by progressive hypertrophy when stimulated with PDGF‐BB. Disaggregated cells from E13.5 mouse testes showed a significant increase in both cell number and DNA synthesis when cultured for 16 h with PDGF‐ BB (100 ng/ml) compared with controls cultured in medium alone (Ricci et al., 2004). 3. Hepatocyte Growth Factor Cell proliferation is induced in dissociated E13.5 mouse testicular cells by HGF; a significant increase was seen in both cell number ( p < 0.001) and DNA content ( p < 0.01) compared with control cells cultured in medium alone (Ricci et al., 2002). Because cell types were not separated in these experiments it is impossible to determine the extent of somatic cell and germ cell contribution to the proliferative eVect, which was also found when cells were labeled with radioactive thymidine. 4. Transforming Growth Factor a TGFa is a member of the epidermal growth factor family and signals through its receptor, epidermal growth factor receptor (EGFR), with eVects on cell proliferation and tissue morphogenesis (Prigent and Lemoine, 1992). Growth of the embryonic rat testis is influenced by TGFa, as shown by

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immunocytochemistry for proliferating cell nuclear antigen (PCNA), although cord formation is unaVected. Treatment of cultured testes with exogenous TGF‐a leads to the proliferation of unorganized cells (Levine et al., 2000a). In TGFa knockout mice there is no alteration in the phenotype of the testis, although when its receptor EGFR is targeted for deletion there is a transient decrease in the relative amount of interstitial cells occurs before birth. Testis growth can be inhibited by the inhibition of EGFR signaling by the EGFR kinase inhibitor. These results indicate that loss of TGFa can be compensated for by other factors (Levine et al., 2000a). 5. Transforming Growth Factor b Family a. Transforming Growth Factor b In their study of TGFb expression in rat testis development (see Section V.A.1), Cupp and coworkers found each isoform showed a diVerent pattern of expression and suggested the three isoforms are diVerentially regulated (Cupp et al., 1999). Testis organ cultures were used to investigate the functional significance of TGFb1 in rat testis development. Urogenital complexes (each composed of a testis and attached mesonephros) were explanted at E13 and cultured on floating filters in the presence or absence of 40‐ng/ml recombinant TGFb1 over 3 days. Seminiferous cord formation was not inhibited in the presence of TGFb1, but the overall size of the testis organ culture was reduced compared with controls cultured in medium alone. A similar reduction in testis growth was seen in E14 organ cultures. One major eVect we had previously noted when explanted E12.5 and E13.5 testes were maintained for 2 or 7 days in the presence of 1‐ng/ml TGFb1, was the more spherical shape which the gonad assumed and which may have a bearing on this size reduction; microscopically there was a distinct increase in the number of cell layers of flattened fibroblasts in the tunica albuginea (Mackay et al., 1995) (Figs. 2 and 3). We also observed good development of the testicular cords which showed an increase in the deposition of collagen fibrils in the extracellular matrix. To investigate the size eVect further, Cupp and coworkers (1999) used a tritiated thymidine incorporation assay: PN0 testis cell cultures were treated with TGFb alone or with positive regulators of PN0 testis growth (FSH, EGF, and 10% fetal calf serum). Treatment with 40‐ng/ml TGFb1 did not significantly alter thymidine incorporation into PN0 testis cultures compared with controls, but did inhibit EGF and FCS‐stimulated thymidine incorporation into PN0 testis cultures, although not FSH‐stimulated thymidine incorporation. Cultures were also subjected to quantitative RT‐PCR to investigate the eVects of EGF and FSH on expression of these TGFb isoforms. Although FSH had no eVect, EGF significantly stimulated expression of TGFb1 and reduced expression of TGFb3 compared with controls (Cupp et al., 1999). In summary, TGFb1 did not prevent cord formation but did inhibit growth of

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FIG. 2 Detail of tunica albuginea from control E13.5 male cultured for 7 div. Superficial layers of fibroblasts (F) are still quite rounded, below cuboidal surface epithelium.

FIG. 3 Experimental male tunica is densely packed and multilayered, consisting of more flattened fibroblasts (F) below a very attenuated surface epithelium.

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the testis in the embryonic and early postnatal periods indirectly, by inhibiting the eVects of the positive growth factor, EGF, which in turn regulated TGFb1 and TGFb3 expression. It is unclear from this study which particular cell type is involved in this inhibition of growth, but the authors suggest that the dramatic reduction in testis size in cultures may result from a reduction in Leydig cell proliferation. Regulation of expression of TGFb1 in the developing testis in vivo may be important both to regulate germ cell numbers initially and later to regulate somatic cell growth (Cupp et al., 1999). In a subsequent study (Konrad et al., 2000), the role of TGFb2 in testicular cord formation has been highlighted (see Section VI.B.3.b). b. Activin Sertoli cell proliferation in cultured testis fragments from PN3 rats has been reported to be significantly increased when FSH is included in the culture medium, but reduced in the presence of activin and follistatin (Meehan et al., 2000). A study using purified proliferating early postnatal rat Sertoli cells has shown that activin A acts directly on PN6 and PN9 (but not on PN3 Sertoli cells), both alone and with FSH to stimulate proliferation. In vivo, peritubular myoid cells may be the source of activin A, as it is secreted at high levels by cultured peritubular cells (Buzzard et al., 2003).

6. Neurotrophic Factors Glial cell line‐derived neurotrophic factor (GDNF) is a distant relative of the TGF‐b superfamily whose receptor GFRa1 lacks a transmembrane and cytoplasmic region and so requires a signaling component, the tyrosine kinase receptor Ret (Massague´, 1996). In the mouse, both GDNF and the related factor neurturin are expressed in the developing urogenital system from E10 to E14 (Golden et al., 1999). Although both sexes express the Ret receptor and low‐level expression of GFRa2, the GDFa1 receptor is highly expressed in the testis but undetectable in the ovary at E14. Although GDNF was highly expressed in the testis at E16 expression of its receptor was undetectable at that stage. Expression of GDNF in the rat testis increases during development reaching a peak at PN7 and declining thereafter (Trupp et al., 1995). Because GDNF mRNA expression is also shown by the mouse Sertoli cell line, TM4 cells, the source of GDNF in the developing testis may be the Sertoli cells (Trupp et al., 1995). In the rat, GDNF produces a marked stimulatory eVect on Sertoli cell proliferation during the early postnatal period and an increase in 3H thymidine incorporation in the presence of FSH (Hu et al., 1999). A proliferative eVect on developing Sertoli cells is also seen in the mouse. Sertoli cells isolated at three stages, E12.5 (the time of cord formation), E13.5 (when gonocytes enter mitotic arrest), and E14.5 (when cords are stabilized)

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FIG. 4 Cultures of E14.5 Sertoli cells after 7 div showing immunopositive staining for PCNA: (A) DMEM alone, (B) DMEM þ 1‐ng/ml NGF, (C) DMEM þ 10‐ng/ml NGF, (D) DMEM þ 100‐ng/ml NGF. Arrows indicate PCNA immuno‐positive cells.

and maintained for 2–7 div show a significant diVerence in proliferation in the presence of GDNF compared with controls (Wu et al., 2005). The neurotrophins, involved in germ cell proliferation (see Section V.A.7) may also play a part in the control of Sertoli cell proliferation. In a preliminary study in our laboratory, mouse E14.5 Sertoli cells were isolated and cultured for 7 div with or without NGF (Fig. 4). A significant increase ( p < 0.001) in cell number was observed with NGF, at all concentrations (1 ng/ml, 10 ng/ml, and 100 ng/ml), compared with controls (Fig. 5A). Furthermore, a significant diVerence in proliferation as measured by PCNA immunocytochemistry was seen in cultures with NGF (at 1 ng/ml and 10 ng/ml, p < 0.001) (Fig. 5B).

VI. Control of Cell Phenotype/Differentiation A. Germ Cell Control One of the most tantalizing problems in germ cell control for many years has been the question of how entry to meiosis is controlled. An important paper has appeared on the role of retinoid signaling in this phenomenon. In an expression screen designed to identify key genes in mouse gonadogenesis, one

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A

Total cell number 200

Total cell number

*** *** *** 100

0 Control

1 ng/ml 10 ng/ml NGF concentration Proliferation

B 50 % PCNA positive cells

100 ng/ml

***

40 *** 30 20 10 0 Control

1 ng/ml 10 ng/ml NGF concentration

100 ng/ml

FIG. 5 Cell number estimates and percentages of proliferative cells with increasing NGF concentrations. (A) Total cell number in cultures with DMEM alone and increasing concentrations of NGF. (B) Percentage of proliferative cells in cultures with DMEM alone and increasing concentrations of NGF. *** p ¼ <0.001.

gene (Cyp26b1) was found to become male sex‐specific by E12.5 and is expressed in developing testicular cords by Sertoli cells and in some interstitial cells (Bowles et al., 2006). The function of this gene is to encode a P450 cytochrome enzyme which degrades retinoic acid (RA), so the source of RA in the developing urogenital system was then investigated and found to be the mesonephroi of both male and female embryos. Using urogenital ridge organ cultures and a variety of molecular markers of meiotic progression,

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exogenous RA was found to stimulate meiotic entry in germ cells, which express both RA receptors and retinoid X receptors at the right time. Evidence that CYP26B1 is the meiosis‐inhibiting substance in males was provided by Cyp26b1 / mouse embryos, in which testicular germ cells expressed Sycp3 (which encodes part of the synaptonemal complex) and Stra8, a premeiotic marker. Knockout ovaries showed an early meiotic progression, indicating early expression of Cyp26b1 may ensure female germ cells do not enter meiosis prematurely. Retinoic acid fulfills all necessary criteria to be identified as the meiosis‐inducing substance; the meiosis‐ preventing substance appears to be an enzyme of retinoid metabolism rather than a secreted signaling molecule (Bowles et al., 2006). 1. Transforming Growth Factor b Family The importance of TGFb family signaling in germ cell control is shown by the expression of its inhibitor, Bambi (Bmp and activin membrane‐bound inhibitor). Significant expression of Bambi mRNA has been shown in the postnatal rat testis by Northern blotting and in situ hybridization. At birth gonocytes in the center of testicular cords show a weak or absent signal, but 5 days later spermatogonia show a readily detectable signal. In the adult rat Bambi mRNA and protein synthesis are predominantly seen in spermatocytes, although signal is also seen in type B spermatogonia and early elongating spermatids. Bambi is therefore likely to be involved in local regulation of TGFb superfamily member activity in a broad spectrum of germ cell types. Sertoli cells of both immature and adult rat testis are also sources of Bambi mRNA (Loveland et al., 2003). a. Bone Morphogenetic Proteins Knockout mice homozygous for the null mutation of Bmp4 have no primordial germ cells (PGCs) and heterozygotes show fewer PGCs than controls as a result of a smaller founding population. This is a result of failure of expression of Bmp4 in the extraembryonic ectoderm prior to gastrulation, which is critical for the specification of the germ cell lineage (Lawson et al., 1999). In addition, Bmp8b is also expressed in the extraembryonic ectoderm in pregastrula and gastrula stage mouse embryos and Bmp8b null mutants show a severe reduction in germ cell number (Ying et al., 2000). Experiments in vitro have shown that BMP4 or BMP8b homodimers alone cannot induce PGC development in murine epiblasts, indicating that the two BMP pathways are required simultaneously for PGC induction. Induction of PGCs in Bmp8b mutants can be rescued by BMP8b homodimers but BMP4 homodimers cannot rescue PGC defects of Bmp4 null mutants; BMP4 proteins may be required for epiblast cells to gain germ‐line competency before the synergistic action of BMP4 and BMP8B (Ying et al., 2001).

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The total number of PGCs is greatly reduced or absent in Smad5 mutant embryos, as in Bmp4 or Bmp8b mutant embryos, demonstrating that Smad5 is an important downstream signal mediator in PGC specification (Chang and Matzuk, 2001). It has also been shown that BMP4‐induced PGC diVerentiation of PGCs from mouse epiblast in vitro is dependent on phosphorylated SMAD1 (Hayashi et al., 2002). Although the role of BMP signaling has been shown to be essential for the diVerentiation of PGCs, the molecular mechanism involved is not fully elucidated. However, direct signaling from the extraembryonic ectoderm to the proximal epiblast is supplemented by an obligatory indirect BMP‐dependent signal via the visceral endoderm (through ALK2, a type I BMP receptor) to induce PGC diVerentiation in the epiblast (Lopes et al., 2004). In a study using recombinant human BMP4 on cultured mouse epiblasts in vitro, the ability to respond to BMP4 signals was acquired between E5.25 and E5.5. Fast acquisition of competence in the proximal epiblast may be controlled by increased expression of Smad1 and the onset of Smad5 expression induced by the extraembryonic ectoderm. Only proximal epiblast cells retain responsiveness to BMP4 for PGC formation at E6.0 and this is associated with expression of Smad5 by the proximal epiblast (Okamura et al., 2005). b. Transcription Growth Factor b In an immunohistochemical study of TGFb1 and TGFb2 expression in rat testis development, from fetal (E19–E21) through neonatal (PN7) and prepubertal (PN21–PN35) to adult (12‐week‐old) stages, TGFb1 was found to predominate in spermatocytes and early round spermatids. However, as spermatids elongated, immunostaining for TGFb1 decreased and became undetectable. At the same time immunostaining for TGFb2, undetectable in spermatocytes and in round spermatids, was very intense as spermatids elongated (Teerds and Dorrington, 1993). The authors suggest two possible functions: First, TGFb may be secreted by germ cells to act in an autocrine manner to control their diVerentiation. Secondly, TGFb released from germ cells may influence neighboring Sertoli cells and may act as a chemotactic agent, either to maintain Sertoli cell cytoplasmic extensions around germ cells or to promote Sertoli cell/ peritubular myoid cell interactions (see Section VI.B.3.b). This study also showed that TGFb1 was present in Sertoli cells throughout development in the rat, with TGFb1 predominating in adult life and TGFb2 immunostaining declining after birth. A similar pattern of expression was seen in Leydig cells, but TGFb immunoreactivity declined before puberty as TGFa immunostaining became intense. This may be related to the fact that TGFb inhibits androgen production by Leydig cells whereas TGFa promotes steroidogenesis (Teerds and Dorrington, 1993). c. Growth DiVerentiation Factor‐9 This member of the TGFb superfamily was identified using degenerate primers corresponding to conserved regions of known family members (McPherron and Lee, 1993). Although initially

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reported to be absent from the testis, growth diVerentiation factor‐9 (GDF‐9) mRNA expression was subsequently discovered in the mouse, rat and human testis using Northern blot analysis, RT‐PCR and in situ hybridization. Expression was seen specifically in large spermatocytes in the later pachytene stage of meiosis I and also in postmeiotic, immature, round spermatids (Fitzpatrick et al., 1998). The role of GDF‐9 in the testis is unclear; it may regulate growth and diVerentiation of other germ cells or Sertoli cells. However, GDF‐9 knockout mice are fertile, so its activity may be compensated for by other TGFb family members (Fitzpatrick et al., 1998). 2. Leptin A product of mature adipocytes, leptin is a 16‐kd peptide hormone that acts as a growth factor in tissues from normal and diseased states (Frankenberry et al., 2004). Expression of its receptor, Ob‐R, was investigated in mouse testes from PN5 to PN30 and in adult testis and brain, using immunohistochemistry. In addition, RT‐PCR and Southern and Western hybridization were used to investigate the presence of mRNA for Ob‐R. At PN5 expression was mainly in type A spermatogonia, whereas at PN20 and PN30 expression was seen in spermatocytes. Only spermatocytes in Stages IX and X of the seminiferous epithelium cycle (stages following sperm release) showed positive expression. As leptin acts through induction of phosphorylation of STAT and mitogen‐activating protein (MAP/ERK), isolated seminiferous tubules were treated with leptin and then phosphorylation of STAT3, ERK1, and ERK2 was examined. Results showed that leptin induces STAT3 phosphorylation in mouse seminiferous tubules and also ERK1, ERK2, and STAT3 phosphorylation in isolated mouse PN5 interstitial cells. The authors postulated that the diVerent downstream results of leptin signaling in spermatogonia and spermatocytes are due to the diVerent Ob‐R isoforms expressed in these two cell types. In spermatogonial stem cells leptin may act through STS3 to prevent diVerentiation, allowing stem cell renewal. However, in the case of spermatocytes, leptin directs cells to full maturation into spermatids instead. The absence of Ob‐R from germ cells in stages other than IX and X of the cycle in adults may be a result of negative feedback regulators from spermatids or other germ cells (El‐Hefnawy et al., 2000). 3. Vascular Endothelial Growth Factor VEGF is involved in angiogenesis in embryonic development and in the mature ovary and uterus during the monthly cycle. Although there is no corresponding cyclical angiogenesis in the adult testis, a great amount of VEGF is produced by the developing testis, localized to Leydig and Sertoli cells (Ergun et al., 1997; Nalbandian et al., 2003). Two of three isoforms of

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the VEGF receptor, VEGFR‐1 and VEGFR‐2 have been shown to be expressed on the surface of Leydig and Sertoli cells, suggesting an autocrine function of VEGF in the testis (Ergun et al., 1997). In an immunohistochemical and RT‐PCR study of the adult mouse testis, strong immunofluorescence for VEGF was seen in interstitial tissue and staining was also observed in Sertoli cells (Nalbandian et al., 2003). In the immature (PN6) mouse testis strong expression of VEGF was observed in Sertoli cells and VEGFR‐1 immunostaining was strong in the interstitial cell population, but was absent from Sertoli cells in this study. Expression of VEGFR‐2 within tubules was localized to type A spermatogonia at this time. Interstitial tissue showed colocalization of VEGF and VEGFR‐2. Immunostaining for VEGFR‐2 was not maintained in the adult testis, although interstitial cells still showed strong immunofluorescence for VEGFR‐2. However, the adult testis showed strong immunofluorescence for VEGFR‐1 in round spermatids and spermatozoa. Although VEGFR‐2 mRNA expression was seen in type A spermatogonia, there was none in pachytene spermatocytes and round spermatids. However, VEGFR‐1 mRNA was expressed in the more advanced forms (pachytene spermatocytes and round spermatids) but not in type A spermatogonia. Moreover, expression of VEGFR‐1 and VEGFR‐2 is inversely correlated during postnatal development of the mouse testis; VEGF produced by Sertoli cells probably exerts a diVerential eVect on proliferation or diVerentiation based on the receptor subtype expressed during spermatogenesis (Nalbandian et al., 2003). 4. Neurotrophic Factors GDNF is said to be essential for regulating the fate of stem cells during spermatogenesis (Sariola, 2001), contributing to the paracrine regulation of spermatogonial self‐renewal in the mouse (Meng et al., 2000). The spermatogonia of mice overexpressing GDNF are unable to diVerentiate, showing a spermatogonial phenotype (Creemers et al., 2002; Meng et al., 2000). Expression of the receptor GFRa‐1 could be used as a marker for undiVerentiated type A spermatogonia (Dettin et al., 2003).

B. Sertoli Cell Control/Testicular Cord Formation 1. Fibroblast Growth Factor 9 In a study of a targeted disruption of FGF9 in the mouse embryo, of 24 E18.5 FGF9–/ embryos examined, 22 had female internal organs (although one showed epididymal‐like tissue as well); of the two phenotypically male knockouts, both showed hypoplastic testes with reduced mesenchyme (Colvin et al., 2001). Ten of 14 phenotypic females proved to be XY on sex genotyping.

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Immunohistochemistry for AMH and in situ hybridization for cholesterol side‐chain cleavage (SCC) cytochrome p450 showed that Sertoli and Leydig cells respectively failed to develop or were lost in most FGF9 / XY gonads. Two FGF9 / XY gonads examined in thin sections showed cell clusters rather than testicular cords; these lacked peritubular myoid cells and showed mesenchymal depletion (Colvin et al., 2001). These results show a clear role for FGF9 in stimulating Sertoli cell diVerentiation and cord formation. EVects on cord formation may result from depletion of mesenchyme and peritubular myoid cells. When isolated E14.5 mouse Sertoli cells are cultured with extracellular matrix (ECM) gel and Fgf9 at a concentration of 10‐ng/ml culture medium, increased proliferation and cordlike aggregation of the cells is seen, with appositional contact of adjacent cell membranes (Willerton et al., 2004). Extracellular matrix includes heparin sulphate proteoglycans that act as low‐aYnity receptors for FGFs and are required to activate FGFRs (Lin et al., 1999; Rapraeger et al., 1991; Schmahl et al., 2004; Yayon et al., 1991). Control cells cultured in medium alone proliferate and attach, but only show minor aggregations (Willerton et al., 2004). Proliferation may be induced in the coelomic epithelium in cultured E11.2– E11.5 XX gonads by FGF9 at 50 ng/ml for 36 h, but this is not suYcient for Sertoli cell diVerentiation and cord formation, indicating that increased proliferation alone is insuYcient for Sertoli cell diVerentiation (Schmahl et al., 2004). 2. Platelet‐Derived Growth Factor The receptor PDGFR‐a can bind PDGF‐A, PDGF‐B, and PDGF‐C homodimers and PDGF‐AB heterodimers. In a study of Pdgfr‐a / mice, E12.5 XY gonads failed to develop normal testis cords and interstitial tissue. A coelomic vessel was present, but showed fewer branches between forming testis cords compared with vessels in control gonads. In a quarter of Pdgfr‐a / mice examined (n ¼ 8), the coelomic vessel was also itself defective. Testis cord formation was delayed; cords had formed by E13.5 but were reduced in number and abnormal in shape (being large and dilated) in Pdgfr‐a / mice (Brennan et al., 2003). The role of PDGF‐BB in testis cord formation was further investigated using a battery of techniques including immunolocalization of PDGF‐BB and PDGF receptors a and b subunits; organ culture approaches utilizing laminin detection, cell migration assay, and reaggregation; Western blot analysis and DNA assay (Ricci et al., 2004). Immunolocalization of PDGF‐BB was seen at a low level in E11.5 male mouse urogenital ridges; at this time, PDGFR‐b subunit positive staining was stronger and restricted to the coelomic epithelium and mesonephric mesenchyme. The PDGF‐a subunit was seen at low levels in some coelomic

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epithelial cells, at the mesonephros‐gonad boundary and less strongly in the mesonephric mesenchyme. Two days later in development, PDGF‐BB appeared in the interstitial compartment, though weakly positive in a large number of cells. Immunostaining for the PDGFR‐b subunit was strong in the coelomic epithelium over the genital ridge, in interstitial cells, and in peritubular cells. Positive staining for the PDGFR‐a subunit was less evident. Male E11.5 urogenital ridges were cultured in medium alone or medium supplemented with PDGF‐BB or HGF. UndiVerentiated male gonads formed cords in the presence of PDGF‐BB, although these were smaller in size than cords formed in the presence of HGF (Ricci et al., 2004). Immunohistochemistry demonstrated the presence of laminin in basement membranes around cords. High doses of the PI3K inhibitor LY294002 totally inhibited cord formation. When disaggregated E13.5 testes were plated on Matrigel‐coated dishes and cultured in the presence or absence of PDGF‐BB at 100 ng/ml, a diVerent reorganization was seen in the presence of growth factor. Larger aggregates were formed, showing a star‐shaped structure rather than the cordlike structures formed following HGF treatments as shown in previous experiments by the same group (Ricci et al., 2002). Once again LY29400 inhibited reaggregation in a dose‐dependent manner. The role of this PI3K inhibitor was first investigated in the developing rat testis, where it was also shown to block cord formation or to reduce the number of testis cords in a dose‐dependent manner in E13 testes in vitro (Uzumcu et al., 2002b). The rationale for its investigation was that the PI3K signal transduction pathway is common to growth factors implicated in testis cord formation, such as NT3, HGF, FGF‐9, and PDGF. 3. Hepatocyte Growth Factor HGF signaling acts via its receptor c‐met to induce epithelial morphogenesis during lung development (Ohmichi et al., 1998). To investigate the role of HGF in mouse testis tubulogenesis (the transition from solid testicular cords to hollow seminiferous tubules), which normally occurs in postnatal life at the same time as the development of Sertoli‐Sertoli tight junctions (Russell et al., 1989), culture experiments were carried out using both isolated primary Sertoli cells from prepubertal mice and an immortalized Sertoli cell line, SF7, established from a PN10 mouse testis (van der Wee and Hofmann, 1999). After 5 div on a Matrigel substrate in culture medium supplemented with 10% fetal calf serum, SF7 cells formed a three‐dimensional (3‐D) network, which proved to be tubular after sectioning. Various growth factors known to be present in Matrigel or serum were investigated; at a concentration of 5‐ng/ml HGF both SF7 cells and primary Sertoli cells formed tubular structures, although higher concentrations caused detachment of cells. Immunocytochemistry showed strong expression of the c‐met receptor in

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both cultured SF7 cells and PG3 peritubular cells. A possible role in vivo was confirmed by reverse transcriptase‐polymerase chain reaction (RT‐PCR) which showed that the HGF gene is transcribed at low amounts in the postnatal and adult testis (van der Wee and Hofmann, 1999). These authors speculated that HGF might be itself regulated by basic fibroblast growth factor (bFGF) as in cultured human mesenchymal cells (Roletto et al., 1996), and that TGF‐b produced by PMCs might be involved in tubule formation by inhibiting HGF‐stimulated branching morphogenesis as in cultured kidney‐derived cell lines (Sakurai and Nigam, 1997). Expression of the HGF receptor, c‐met, was also shown by in situ hybridization in embryonic male gonads at E12.5, when testis cords first appear. A day earlier expression was restricted to the mesonephros, and at E13.5 higher expression was seen in testicular cords (Ricci et al., 1999). In culture experiments, serum addition was found to be essential for testis diVerentiation from indiVerent urogenital ridges, but HGF added alone to culture medium in the absence of serum was suYcient to allow cord development (Ricci et al., 1999). However, others have found mouse testis diVerentiation can proceed in the absence of serum in vitro from the indiVerent stage (Mackay and Smith, 1986, 1989). Northern blot analysis showed strong male‐specific expression of HGF in E13.5 and E15.5 mouse testes. Immunohistochemistry was used to determine the precise localization of expression, which was found in cells of the tunica albuginea, the interstitial compartment, and in peritubular myoid cells. Expression was seen in the coelomic epithelium and in small groups of cells within the genital ridge in E11.5 male urogenital complexes; strong expression was also seen in the mesonephric mesenchyme (Ricci et al., 2002). Culture experiments showed that dissociated E13.5 testes formed cordlike structures in the presence of HGF (5–100 U/ml). At the highest dose of HGF 3‐D networks were formed on the Matrigel substrate; these cords were longer and wider than those occasionally observed in control cultures (Ricci et al., 2002). 4. Transforming Growth Factor b Superfamily a. Anti‐Mu¨llerian Hormone When rat prospective ovaries are explanted at E14 and cultured for 3–7 div with purified bovine AMH, there is a decrease in gonadal volume, germ cell depletion and diVerentiation of cells resembling rat fetal Sertoli cells (Vigier et al., 1987). Sertoli cell diVerentiation may simply be a result of the germ cell depletion, because follicle cells can transdiVerentiate as Sertoli cells if germ cells are lost after entry to meiosis (MacIntyre, 1956; McLaren, 1991). In vivo, AMH is first expressed in mouse pre‐Sertoli cells at E12.5, when testicular cords are forming. Expression declines between 2 and 3 weeks postnatally, at the time when male germ

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cells enter meiosis, suggesting a role for AMH in control of entry to meiosis (Mu¨nsterberg and Lovell‐Badge, 1991). This is also the time of development of the blood‐testis barrier, which results in a higher AMH concentration in the seminal plasma than in blood (Rey et al., 2003). Further, laminin a‐5 reappears at this time in the basement membrane of the seminiferous tubules (Pelliniemi and Fro¨jdman, 2001). Transgenic ‘‘knock‐in’’ mice have been produced that chronically express human AMH under the control of the mouse metallothionein‐1 promoter (Behringer et al., 1990). Mu¨llerian duct diVerentiation was inhibited in females chronically expressing AMH, no uterus or oviducts were seen and at birth the ovaries had a reduced number of germ cells. These germ cells were subsequently lost over the first 2 postnatal weeks and the somatic cells reorganized into structures resembling seminiferous tubules, which had disappeared in adult females. Although the majority of transgenic males developed normally, in the two lines with the highest levels of AMH expression some males showed impairment of mesonephric duct development, undescended testes with no germ cells, and feminization of the external genitalia (a vaginal opening and mammary gland development). These results may be explained by the fact that high levels of AMH aVect Leydig cell development in the testes of these animals, resulting in inhibition of androgen biosynthesis. Similarly, human recombinant AMH has been shown to inhibit LH‐stimulated testosterone production by fetal rat Leydig cells in vitro, in a dose‐dependent manner (Rouiller‐Fabre et al., 1998). Regarding failed testicular descent in AMH transgenic males, the first phase of testis descent is androgen‐independent, controlled instead by AMH; high levels of AMH may lead to a downregulation of its receptor on cells controlling testis descent (Behringer et al., 1990). Ovarian development could occur when AMH levels were suYcient to inhibit Mu¨llerian duct development, suggesting that a higher level of expression is required for the ovarian eVect (Behringer et al., 1990). Further evidence for this idea was provided earlier when E14.5 rat ovaries were cultured with medium conditioned by the preliminary culture of testes from young or fetal rats. In these ovaries follicles were rare, germ cell degenerated, and cords like seminiferous cords developed. Bioassay culture of genital ducts with transformed ovaries showed AMH was produced, but no germinostatic activity (i.e., suppression of oogonial proliferation) on cocultured E13.5 ovaries was seen (Pre´pin and Hida, 1989), as is exerted by isolated fetal testis seminiferous cords (Pre´pin et al., 1985). Perhaps suYcient AMH was generated from transformed ovaries for the anti‐Mu¨llerian eVect, but not enough for the germinostatic eVect. In our own work in the mouse, we have observed a loss of germ cells in E12.5 ovaries cocultured with Sertoli cells isolated at the same age, with no evidence of the remaining germ cells entering meiosis (Mackay et al., 2004b). If ovaries were explanted a day

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FIG. 6 Mouse Sertoli cell culture after 7 div in the presence of 10‐ng/ml GDNF. Immunofluorescence for AMH (red), a marker for Sertoli cells and for a‐smooth muscle actin (green), a marker for peritubular myoid cells.

later, however, meiotic germ cells survived when cultured together with Sertoli cells although the ovigerous cords did display signs of masculinization. The presence of AMH (Fig. 6) was demonstrated in our Sertoli cultures by immunocytochemical labeling (Mackay et al., 2004b). b. Transforming Growth Factor b To investigate the functional role and possible involvement of TGFb2 in mediating epithelial/mesenchymal interactions in the developing rat testis, TGFb2 secretion in vitro in monocultures and cocultures of PN19 (mesenchymal) peritubular cells and (epithelial) Sertoli cells has been determined, using a highly sensitive ELISA (Konrad et al., 2000). Peritubular myoid cells and cocultures secreted increasing amounts of TGFb2 in the first week of culture, although Sertoli cell secretion was only marginal. The total amount of TGFb2 in cocultures on the first 2 days was similar to that of peritubular cell cultures, but became reduced from 3 div. Newly synthesized TGFb cannot interact with TGFb receptors until it has been activated by proteolytic cleavage. Secretion of bioactive TGFb2 was highest in cocultures and showed a small peak on day 2,

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probably preceding the formation of Sertoli cell aggregates, which appeared after 3 div. Sertoli cell aggregation or tubule formation was increased by a factor of two after stimulation with recombinant TGFb2 in comparison with monocultures. These results, together with the fact that TGFb2 has been found in other regions of active morphogenesis involving epithelial‐ mesenchymal interactions (Konrad et al., 2000; Millan et al., 1991), support a similar role in the developing testis; TGFb2 may mediate the Sertoli cell/peritubular myoid cell interactions that underlie cord formation. 5. Neurotrophic Factors A reduction in testicular cord number is seen in trkC knockout mice at E14 and in cord area at E19; similarly trkA knockouts show a reduction in cord number at E14. Further, in both trkA and trkC knockout mice development is delayed at E13 (Cupp et al., 2002). a. Neurotrophins The role of neurotrophins in testicular morphogenesis has been investigated in the rat (Levine et al., 2000a), in which organ cultures have been treated with an inhibitor (K252a) to the high‐aYnity receptor, trk. In cultures explanted at E13 (i.e., prior to cord formation in the rat), testicular cord formation is completely inhibited, whereas no alteration is seen in cultures explanted at E14 when cords are already present. Null mutant mice for NT3 show normal morphology at both E15 and E17 as do trkC null mutants. However, both mutants show less interstitial tissue than wild‐type animals, which may be a result of impaired migration from the mesonephros (see Section III.B.4). Expression of the low‐aYnity neurotrophin receptor p75/LNGFR is seen in E13 gonads of both sexes and then around cords in the testis alone at E14, although expression reappears in the ovary at the time of follicle development from E16 to E19 (Levine et al., 2000a). b. Glial Cell Line‐Derived Neurotrophic Factor Mouse Sertoli cells isolated at E13.5 and cultured in extracellular matrix‐coated wells form obvious cordlike aggregations after 48 h; when cells are isolated at E12.5, the time of cord formation in vivo, aggregation of Sertoli cells (showing apposition of cell membranes at more than one surface) is observed after only 1 div. Fewer cordlike aggregations are seen in the absence of exogenous GDNF (Wu et al., 2005).

C. Leydig Cell Control The signaling molecule Desert hedgehog (Dhh) expressed by Sertoli cells is necessary for Leydig cell diVerentiation (Clark et al., 2000; Yao et al., 2002). Evidence from double mutants for the orphan nuclear receptors Sf1/Dax 1

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suggests they function cooperatively to enhance Dhh expression (Park et al., 2005). Fetal Leydig cell markers (Cyp17 and Cyp11a1) show reduced expression in heterozygous Sf1‐deficient mice at E13.5, consistent with dose‐ dependent eVects of Sf1, similar to those seen in humans (Achermann et al., 2002). 1. Platelet‐Derived Growth Factor Homozygous mutant mice for the gene encoding PDGF‐A die postnatally of pulmonary failure, but some individuals survive long enough for eVects on the testis to be studied. Null mutant mice weigh less than wild‐type littermates and show an even more pronounced testicular size reduction. Numbers of Leydig cells are progressively reduced in the postnatal period, being almost completely absent by PN42. A lack of both bromodeoxyuridine (BrdU) labeling and TdT‐mediated dUTP biotin nick end labeling (TUNEL) show the low number of Leydig cells is likely a result of proliferation arrest rather than an increase in apoptosis (Gnessi et al., 2000). The authors suggest that in the absence of PDGF‐A the normal pubertal replacement of the fetal Leydig cell population by adult cells is deranged as adult Leydig cell precursors fail to proliferate and diVerentiate. The ensuing reduction in testosterone would then cause the spermatogenic arrest and germ cell degeneration seen in the mutant mice. In their study of Pdgfr‐a / mice (see earlier), Brennan et al. (2003) found that expression of the Leydig cell‐specific marker P450 side chain cleavage (Scc) was at much lower levels (if expressed at all) in Pdgfr‐a / mice compared with wild‐type controls, reflecting impaired development of the fetal Leydig cell population. In coculture experiments using gonads and GFP‐labeled mesonephroi, when the gonad was Pdgfr‐a / there was no Leydig cell diVerentiation, even if the mesonephros was wild‐type. Because Dhh signaling is necessary for fetal Leydig cell development (Yao et al., 2002), Dhh and Pdgfr‐a and Pdgf‐A expression were investigated by in situ hybridization. Although wild‐type E11.5 gonads show Dhh expression, none was seen in Pdgfr‐a / mice at this time. However, by E12.5 Dhh expression in Pdgfr‐a / mice was similar to that in controls although expression of the Dhh receptor Ptch1 was still reduced at E13.5. Because Ptch1 is upregulated in cells exposed to DHH, Pdgfr‐a may act with Dhh to promote the expansion and/or diVerentiation of Ptch1‐positive cells. This could be a result of defects in proliferation changing the number of Ptch1 precursor cells, or less directly through structural and endothelial defects in Pdgfr‐a / gonads interfering with the cues needed to specify Leydig cell fate (Brennan et al., 2003). An attempt was made in this study to alter the diVerentiation of XX gonads; although exogenous PDGF could induce migration and upregulation of Pdgfr‐a in XX gonads in vitro, Leydig cell diVerentiation was not seen.

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The authors speculate that this could be due to the presence of female factors repressing Leydig cell development such as WNT4, which has been shown to repress steroid cell development in the developing ovary (Vainio et al., 1999).

2. Fibroblast Growth Factors In an immunohistochemical study to investigate expression of FGF receptors (FGFRs) in the rat testis, a change in expression of FGFRs was found in the fetal Leydig cell and during development of the adult Leydig cell population. Both adult and fetal Leydig cells express FGFR‐1, but immature adultlike Leydig cells diVer in also expressing FGFR‐2, FGFR‐3, and FGFR‐4. However, adult Leydig cells do not express FGFR‐3, which may therefore be a specific functional requirement for the immature adultlike Leydig cell population (Cancilla and Risbridger, 1998).

D. Peritubular Myoid Cell Control 1. Platelet‐Derived Growth Factor When PMCs are isolated from 17‐day‐old rats and cultured in vitro in serum‐ free medium, they assume a round shape and are small in size, although they still express PMC markers such as desmin and vimentin. At isolation they do not show PDGF‐binding sites, although after a day in vitro in serum‐free conditions, high‐aYnity PDGF receptors induced by cell culturing can be detected. If then treated with 1.6‐nmol PDGF‐AA, PDGF‐BB, or PDGF‐ AB, the cells show a fibroblast appearance with elongated slender processes and retracted cell bodies, that is, they regain their characteristic PMC phenotype. Expression of the PMC structural phenotype is accompanied by functional activity, because PDGF also increases the release of matrix components: type IV collagen and fibronectin (Gnessi et al., 1993). Smooth muscle a‐actin (Sma‐actin) filaments become reorganized as stress fibers after 24 h stimulation with PDGF‐BB; morphological changes and altered distribution of Sma‐actin within PMCs are seen at a PDGF concentration as low as 10 ng/ml (Chiarenza et al., 2000). To test the hypothesis that PDGFs and PDGFRs are expressed during testicular cord formation and that inhibition of their action influences normal cord development, rat embryonic testis cultures were cultured for 3 days with PDGFR‐specific tyrosine phosphorylation inhibitors (the tyrphostins, AG1295 or AG1296). Tyrphostin‐treated testes formed abnormal swollen and fused cords, perhaps as a result of an alteration in mesonephric cell diVerentiation (Uzumcu et al., 2002a), to form peritubular myoid cells.

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2. Neurotrophins Precursors of the peritubular myoid cell population can be identified by the presence of the low‐aYnity p75/NTR neurotrophin receptor. They can be isolated from E12.5 mouse mesonephroi and will diVerentiate in vitro to peritubular myoid cells. Immunohistochemistry shows a progressive occupation of the interstitial tissue by p75/NTR positive cells between E10.5 and E12.5 and postnatal testis sections show peritubular cells coexpressing p75/NTR and/or smooth muscle actin (Campagnolo et al., 2001).

VII. Experimental Manipulations In Vitro The existence and role of putative growth factors in testis diVerentiation has been investigated by a variety of experimental techniques in vitro. Culture systems allow continued development while environmental conditions are varied to investigate possible eVects on diVerentiation. There are certain limitations however: if gonads are removed from a mouse embryo on E10 they will not diVerentiate, even with serum present (Taketo and Koide, 1981). If gonads are removed a day later on E11 serum must be added to the culture medium to allow diVerentiation in vitro, but from E12 onward gonads will continue to grow in culture medium without serum, diVerentiation being directed by their genetic sex (Taketo et al., 1986). There is no qualitative morphological or functional diVerence between diVerentiation achieved in vitro compared with that in vivo, although there is a slight delay in vitro, presumably a result of the trauma of explantation (Mackay and Smith, 1989). DiVerent culture systems have been utilized to test the eVect of male factors on female gonads and vice versa. Byskov and Saxe´n (1976) used a transfilter approach in an attempt to test the presence of diVusible factors. They reported the induction of meiosis in genetically male indiVerent (E11) gonads by older (E14) ovaries separated from them by a Nuclepore filter. When older testes (E14) and ovaries of the same age were cultured together but separated by a filter, meiotic germ cells present in the ovary were arrested before entering the diplotene stage. The authors argued for the existence of meiosis‐inducing and meiosis‐preventing substances produced by the female and male gonads respectively. However, the interpretation of this experiment was qualified by a later demonstration that microscopical cell processes could cross the filter (Lehtonen et al., 1975; Saxe´n et al., 1976). Burgoyne and coworkers also used a transfilter approach to culture E11.5 XX and XY indiVerent mouse gonads together, and concluded diVerentiation proceeded according to genotype. However, as these authors pointed out, the development of the embryonic

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testes was poor, so the absence of a masculinizing influence was not entirely convincing (Burgoyne et al., 1986). In our laboratory we cultured indiVerent E11 mouse gonads together in mixed sex groups for up to a week and found no inhibition of one sex by the other; however, on the whole ovaries developed further in culture than testes (Mackay and Smith, 1986). This lack of either meiotic triggering or inhibiting eVects may be explained by the fact that such factors act within a limited radius of activity. More than thirty years have elapsed since Byskov and Saxe´n proposed the existence of meiosis‐inducing and meiosis‐preventing factors. A prevailing view has been that all germ cells are programmed to develop as oocytes, with the timing of meiotic entry a cell‐autonomous event rather than an induced response (McLaren, 2003; McLaren and Southee, 1997; Ohkubo et al., 1996), obviating the need for a meiotic‐inducing factor. Female germ cells of E12.5 or younger can be inhibited from entering meiosis if aggregated with E12.5 male genital ridge cells, indicating that entry to the spermatogenic pathway is an induced response (Adams and McLaren, 2002), dependent on a meiotic inhibitor. When E11.5 mouse male genital ridges are cultured without their associated mesonephroi, germ cells develop as prespermatogonia even though the diVerentiated Sertoli cells do not enclose them in cords (Buehr et al., 1993b). This finding suggests the meiotic‐inhibiting factor may be produced by the Sertoli cells, but does not depend on enclosure of germ cells within cords. Possible candidates have been identified (McLaren, 2003) as prostaglandin D2 (Adams and McLaren, 2002) and the product of a novel gene, Tdl (testis‐specific b‐defensin–like gene). The latter shows Sertoli cell‐specific expression and sequence homology to the antimicrobial peptides b‐defensins (Yamamoto and Matsui, 2002). However, a paper cited earlier (see Section VI.A) shows that there is indeed a meiosis‐inducing factor, retinoic acid, and it is controlled by an enzyme of retinoid metabolism, CYP26B1, the most likely meiosis‐preventing substance (Bowles et al., 2006). A body of work has been carried out in the rat using a variety of in vitro techniques to investigate the role of AMH (see Section VI.B.3.a). When E14.5 rat ovaries are cultured on either side of a single E17.5 testis masculinization of the ovary is produced, with the presence of testicular cords and AMH production, but only if the gonads are in contact and only when E17.5 testes (which exhibit a strong Mu¨llerian‐inhibiting activity) are used (Charpentier and Magre, 1990). These results suggest a role for AMH in functional masculinization of fetal ovaries in vitro in the rat; however, the possibility that testicular cells have simply migrated into the ovaries cannot be excluded. A further finding to emerge is that a ‘‘germinostatic’’ factor diVerent from AMH is produced by fetal or postnatal rat testes and reduces the number of germ cells in E13.5 ovaries after 4 div (Charpentier and Magre, 1989; Pre´pin et al., 1986) or in E14.5 ovaries after 12 div (Pre´pin and Hida, 1989).

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The culture environment of explanted gonads may be manipulated in a number of experimental paradigms. One with which we have generated some interesting results is the maintenance of either ovaries or testes, from a number of diVerent developmental ages, in medium which has been previously conditioned by the presence of gonads from the opposite sex. When E13 ovaries were cultured for 4 days in medium which had been conditioned for 2 days previously by the presence of E13 testes (generating E13–E15 testis‐CM) the mean number of oocytes in the explanted ovaries had dropped by nearly 50% (713 177 as opposed to 1218 166 in cultured control explanted ovaries, p < 0.05); this germinostatic eVect, similar to that reported for the rat (see earlier) was eliminated if the testis‐CM was heat‐inactivated (Tavendale et al., 1992). Germ cells were shown by TEM to have reached a meiotic equivalent to the E17 stage, so that although numbers were reduced those surviving continued to diVerentiate along the female path. It was proposed that AMH might be a candidate causing this, especially as our later work demonstrated that E12.5 (although not E13.5) ovaries maintained in the presence of Sertoli cells isolated at a time when they are producing AMH showed a similar eVect (Mackay et al., 2004b). Electrophoretic analysis of the testis‐CM however, demonstrated the presence of proteins (absent from E13 to E15 ovary‐CM) with molecular weights higher than that of AMH (140 kDa), indicative that other putative factors were responsible (Tavendale et al., 1992). In parallel experiments testes were cultured in ovary‐CM for similar time periods. In E13.5 and E14 testes maintained in E15–E17 ovary‐CM there were no signs of germ cells entering meiosis (Fig. 7), but a significant reduction in the area occupied by the testicular cords in experimental, compared to control, cultured testes was evident (29.7 1.32% in experimental testes compared to 22 1.23 in gonads maintained in normal unconditioned medium p < 0.05). There was a concomitant increase in the amount of interstitial tissue, whereas in the cords small Sertoli cells with irregularly shaped nuclei were located peripherally enclosing the large pale germ cells (Figs. 8 and 9). The WolYan Duct was well maintained in experimental E14 testes cultured in E15–E17 ovary‐CM, however the Mu¨llerian duct showed typical signs of involution (Fig. 10). Another useful technique is that of disaggregation/reaggregation which can be applied to test the importance of control factors in diVerentiation. Cells have been disaggregated from newborn rat testes and allowed to reaggregate in rotation cultures where they reaggregated to form testicular tissue after 25 hours (Grund et al., 1986). A disaggregation‐reaggregation culture technique has also been used to show the E11.5 male genital ridge produces a factor inhibiting germ cell entry to meiosis; prior disaggregation of the genital ridge impairs cord formation at this stage (although not at E12.5) and disrupts its production (McLaren and Southee, 1997). Mouse gonads dissociated at

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FIG. 7 Electron micrograph of experimental E14 testis cultured for 4 div in E15–E17 ovary‐ CM shows detail of testicular cord. Centrally located germ cell (G) shows no evidence of meiosis. A basal lamina (arrow) is present around the developing testicular cord.

FIG. 8 E14.5 control testis cultured 4 div. Note tunica albuginea (TA), well‐organized testicular cords (TC) with centrally placed germ cells and developing Leydig cells (L) within the interstitium.

E13.5–E14.5 will reorganize in vitro but their reaggregation is prevented by the inclusion of antibodies to laminin or the a6 subunit of its integrin receptor (Pesce et al., 1994). In our laboratory a similar approach has been used to show

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FIG. 9 Testis removed at E14 and cultured for 4 div in E15–E17 ovary‐CM. Tunica albuginea is present (TA). Testicular cords appear reduced in size and interstitial tissue increased in volume. DiVerentiated Leydig cells (arrow) lie within the somatic tissue.

FIG. 10 WolYan and Mu¨llerian duct associated with one experimental E14.5 testis cultured 4 div in E15–E17 ovary‐CM. The WolYan duct (W) is well‐maintained whereas the adjacent Mu¨llerian duct (M) shows signs of involution such as an epithelial cuV (arrows).

the functional importance of E‐cadherin in gonadal development, dissociating and culturing E17 gonads in the presence and absence of antibody to E‐cadherin (Mackay et al., 1999). This in vitro technique (dissociation followed by reaggregation in the presence or absence of neutralizing antibodies against

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the factor of interest) oVers a useful adjunct to the mouse knockout model, especially if the gene in question has housekeeping functions when overall development may be compromised (Mackay et al., 2004b). VIII. Concluding Remarks DiVerent approaches have been applied to investigate the role of growth factors in testis development. One is to screen knockout gene mutants for eVects on testis development, another is to examine the developmental steps involved in testicular morphogenesis and to hypothesize which growth factors might be involved, based on findings in other systems. Culture approaches provide a means of creating knockout equivalents, by culturing in the presence of neutralizing antibodies. Possible cell and tissue interactions can be investigated in vitro and occasionally diVusible signals are found by this approach which can then be identified, although in the case of the meiosis‐inducing and meiosis‐preventing substances this has taken 30 years. Genes encoding growth factors of interest can be silenced by means of small interfering RNAs (siRNAs), a relatively new technique that has proved to be a powerful and widely used tool for the analysis of gene function in mammalian cells (Haraguchi et al., 2004). Viral‐mediated delivery of siRNA specifically reduces expression of targeted genes in various cell types, both in vitro and in vivo (Xia et al., 2002); siRNA technology can also be applied in organ culture experiments (Davies et al., 2004). Other genetic approaches include expression screens which can be applied to discover new genes that are sex‐ specifically expressed during mouse gonadal organogenesis (Bowles et al., 2006; Nordqvist and Tohonen, 1997; O’Shaughnessy et al., 2003). Such tools will prove useful in the future as alternatives to creating null mutant mice. Summarizing the evidence presented here for the importance of growth factors in morphogenesis of the testis, some can be seen as key players, active in several diVerent roles at diVerent times (Table I). The PDGF/PDGFR system has been highlighted as a major factor in testis morphogenesis (Brennan et al., 2003; Mariani et al., 2002; Puglianiello et al., 2003), mediating testis cord development and fetal Leydig cell development, with a possible role in the proliferation and migration of PMC precursors from the interstitial tissue to the peritubular area. PDGF‐A/PDGFR‐a interactions also drive precursors to commit to the adult Leydig cell phenotype (Mariani et al., 2002). FGF9 is a key factor acting downstream of Sry controlling mesonephric migration, and the proliferation, aggregation and diVerentiation of Sertoli cells as well as promoting XY germ cell survival (Colvin et al., 2001; DiNapoli et al., 2006; Willerton et al., 2004). Furthermore, there is increasing evidence for a significant role for neurotrophic factors in testis development (Cupp et al., 2000, 2002, 2003; Levine et al., 2000b; Wu et al., 2005).

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GROWTH FACTORS AND TESTIS DEVELOPMENT TABLE I Summary of Growth Factors Involved in Testicular Morphogenesis Event

Growth factor

Function, species

Migration Germ cells

TGFb1 SCF SDF1 FGF2

Mesonephric cells including PMCs, endothelial cells

TGFb3 PDGF HGF AMH Neurotrophins

Chemotropic factor, mouse Migration, mouse Migration, mouse Shape changes during migration, mouse Induces migration, rat Shape changes during migration, mouse, rat Increases migratory activity, mouse Induces migration in XX, E11.5 mouse Migration, mouse, rat

Vascular Development VEGF

Mouse, blocked in XX gonad by Fst and Bmp2 acting downstream of Wnt4

TGFb

" Apoptosis or# proliferation, mouse, rat " Spermatogonia, rat " Proliferation and survival, mouse " Proliferation, mouse " Proliferation, mouse, rat " proliferation, PN rat " Survival, proliferation, mouse " Survival, rat Leydig cell growth inhibitor, rat Survival factor, rat Sertoli cells Sertoli cell proliferation, mouse PMCs proliferation, rat " proliferation, PN Sertoli cells, rat " proliferation, Sertoli cells, rat, mouse " proliferation, Sertoli cells, mouse

Proliferation Germ cells

Somatic cells

Activin (þFSH, Fst) SCF LIF FGF2 PDGF GDNF Neurotrophin TGFb1 FGF2 FGF9 PDGF Activin (þFSH) GDNF NGF

Control of Cell Phenotype Germ cells

BMP4, BMP8b TGFb1 TGFb2 Leptin VEGF GDNF

Specification of germ cell lineage Expressed in spermatocytes, early round spermatids, rat Intense expression as spermatids elongate ?Stem cell renewal, mouse Proliferation or diVerentiation, mouse Stem cell renewal, mouse (continued)

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TABLE I (continued ) Event Sertoli cells/cord formation

Growth factor TGFb2 AMH FGF9 PDGF HGF GDNF

Leydig cells PMCs

Neurotrophins Pdgf‐a Pdgf Neurotrophin

Function, species Sertoli cell/PMC interaction in cord formation, rat ? Cord formation, mouse Sertoli cell diVerentiation, cord formation, mouse Cord formation, mouse Cord formation, mouse Cordlike aggregation of Sertoli cells, mouse Cord formation in e13 rat Leydig cell diVerentiation and proliferation, mouse Phenotype Mouse PMC precursors express receptor p75/ntr

TGF, transforming growth factor; SCF, stem cell factor; SDF1, stromal cell-derived factor 1; FGF, fibroblast growth factor; PDGF, platelet‐derived growth factor; HGF, hepatocyte growth factor; AMH, anti‐Mu¨llerian hormone; VEGF, vascular endothelial growth factor; Wnt4, gene controling female differentiation; FSH, follicle stimulating hormone; Fst, follistatin; LIF, leukemia inhibitory factor; GDNF, glial cell line‐derived neutrotrophic factor; PN, postnatal; PMC, peritubular myoid cells; NGF, nerve growth factor; BMP, bone morphogenetic hormone; p75/ntr, neurotrophin receptor; ?, possible role in; ", increases; #, decreases.

It looks as if there is not just one key growth factor involved in testis development but several interchangeable growth factors and their family members, which is not surprising as this would provide a fail‐safe mechanism in the event of gene damage. Ricci et al. (2004) suggest some of the factors involved in the regulation of migration of cells from the mesonephros and testicular cord formation converge to a common signaling pathway, the P1–3K pathway. This could explain the lack of a severe testicular phenotype in knockouts for c‐met (Bladt et al., 1995; Ricci et al., 2002), PDGFR‐b (Soriano, 1994), trkA, and trkC neurotrophin receptors (Cupp et al., 2002). Although little sequence similarity is found between the growth factors, when a comparison is made of the crystal structures of TGF‐b2, PDGF‐BB, and NGF, a common structural motif is seen involving two pairs of b‐strands and six conserved cysteine residues arranged as a ‘‘cysteine knot’’ (McDonald and Hendrickson, 1992). One other cysteine residue forms a single disulfide bridge between the two subunits, forming a covalently linked dimer, critical for biological activity (Shimasaki et al., 2004). Therefore, although these growth factors show little sequence similarity and diVerent dimerization, they nevertheless have a similar protomeric organization (Wall and Hogan, 1994). Much remains to be elucidated about the events downstream of Sry expression. Problems remaining to be solved at the time of writing include

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Germ cells

Proliferation and differentiation

Cadherin α

Proliferation

b

Sertoli cells

Growth factors (e.g., PDGF, FGF GDNF, NGF)

AMH

Wnt signaling

Differentiation

FSH Basement membrane

Growth factors P-Mod-S

αb Dhh

Integrins

FGF9-heparin sulphate complex

Dhh

FN LAM

ECM effects

?

Peritubular myoid cells

LH

Leydig cells

Differentiation Testosterone

Differentiation

FIG. 11 Somatic and germ cell interactions in the developing testis.

the origin of the Leydig cell population and the significance of the diVerent timing of tunica albuginea development in the two sexes. However, our understanding of the way in which the indiVerent gonad is influenced to develop along male lines has been greatly improved since the discovery of Sry. Deciphering the role of growth factors and the other extrinsic developmental cues, together with the resulting signaling cascades which potentially regulate cell proliferation and further diVerentiation, has increased our appreciation of how the interactions between the respective cell types within the testis ensure development proceeds successfully (Fig. 11). Acknowledgments We are grateful to the Wellcome Trust for their financial support of some of the work included here (Grant number 067482).

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Flagellar Length Control in Chlamydomonas—A Paradigm for Organelle Size Regulation Kimberly A. Wemmer and Wallace F. Marshall Department of Biochemistry, University of California, San Francisco, San Francisco, California 94158

A fundamental unsolved question in cell biology is how the cell controls the size of its organelles. Cilia and flagella are an ideal test case to study the mechanism of organelle size control, because their size is easily measured and can be represented by a single number—length. Moreover, the involvement of cilia in many developmental and physiological processes suggests an understanding of their size control system is critical for understanding ciliary diseases, many of which (e.g., autosomal recessive polycystic kidney disease) are known to involve abnormally short cilia. The flagella of the model organism Chlamydomonas reinhardtii provide the best genetic and cell‐biological system to study length control of cilia. Studies in this organism using genetics, biochemistry, imaging, and mathematical modeling have revealed many genes involved in length control of cilia and flagella, and have suggested several testable models for length regulation. KEY WORDS: Primary cilia, Feedback control, Intraflagellar transport, IFT, Organelle abundance, Homeostasis, Noise, Nanotechnology. ß 2007 Elsevier Inc.

I. Introduction Great leaps in understanding cell biology have been occurring, yet we have only begun to understand the importance of organelle size control for the optimal functioning of cells. The organelles of a cell must be the correct size to perform their required functions or the biology of the cell will break down. In addition, organelle size also plays an important role in cell diVerentiation International Review of Cytology, Vol. 260 Copyright 2007, Elsevier Inc. All rights reserved.

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and identity, with diVerent cell types varying a great deal in their requirement for and use of organelles to perform their specific functions. The study of organelle size control will be crucial to a complete understanding of how cells function. In addition to being able to regulate the overall size of the cell body (Morris, 2002; Umen, 2005), cells must have a way to control the abundance or quantity of each organelle within the cell. For most organelles, the abundance in a given cell will be a function of the number of individuals of each organelle present, and the size of each organelle. Depending on how size and number aVect function, the cell might be more interested in controlling the size of individuals, or alternatively it might be more important to control the total abundance regardless of how this material is apportioned among the multiple copies of the organelle found within one cell. Flagella and the centrioles that nucleate them provide a very convenient approach to the study of organelle abundance, because they separate the two factors of number and size. The number of flagella in the cell is determined entirely by the number of centrioles that become active as basal bodies, and so flagellar abundance can be expressed strictly in terms of the size of the flagella. Conversely, centrioles are always the same size, and hence their abundance can be expressed strictly in terms of the number of centrioles present. Taken together, the centriole‐ flagella system allows the general problem of organelle abundance to be reduced into two distinct problems of size and number. It also turns out that flagella have special advantages as a system for the study of size, even apart from the fact that number need not be taken directly into consideration as it would for other organelles. To see this advantage, we first discuss an overview of organelle size control systems, before moving on to a summary of the specialized features of flagella that relate to size.

II. Size of Organelles A. Size Control 1. Examples of Studies of Organelle Size Control Very few studies of the mechanisms that determine size in eukaryotic organelles have been done. Size control has been studied for several viral and prokaryotic systems, especially bacteriophage tails, bacterial flagella, and flagellar hook structures. In these cases, identification of mutants aVecting length has played a key role in suggesting possible mechanisms for length control. For instance, in bacteriophage, mutants in specific proteins result in defined reductions in length proportional to the size of the deleted region,

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suggesting the gene products function as molecular rules (Katsura, 1990). In bacteria, length control of hooks and flagellar filaments has been studied by both genetic and math modeling approaches (Keener, 2006), resulting in a fairly detailed understanding of size control. However, these structures are exceedingly small, and one can legitimately ask whether the types of control systems that have evolved to regulate such small sizes can also work in the much larger organelles of eukaryotes. The majority of cellular organelles are membrane‐bound compartments with potentially complex three‐dimensional (3‐D) structures. The size of organelles tends to be consistent within a given cell type, and moreover is under a degree of cell‐cycle dependent regulation (reviewed in Blank et al., 2006). The endoplasmic reticulum (ER) serves as an excellent example. Although the structure is challenging to measure, an important insight has been gained from studies of the unfolded protein response (UPR), a molecular pathway that becomes activated when the ER is unable to properly fold proteins within its lumen. Activation of the UPR pathways causes induction of a large number of genes, some of which encode chaperones and other response proteins that directly cope with the unfolded proteins, but more interestingly, some of the UPR targets appear to be genes involved in ER biogenesis. Research has suggested UPR plays a normal role in controlling ER size, using folding of proteins eVectively as a size sensor (Bernales et al., 2006). The idea is, assuming secreted proteins are produced at a constant rate, then if the ER were to become too small to cope with these proteins, the UPR would trigger additional ER synthesis until the organelle became large enough to perform its task. This is an interesting system in which the organelle does not necessarily attempt to reach a defined size, but just a defined level of functionality depending on the particular requirements of the cell. This model suggests many interesting surprises may await us as we probe more deeply into the mechanisms controlling organelle size. 2. Flagella as a Model System for Size Control However, this fascinating problem can be technically diYcult to study, as determining the size of organelles is a very diYcult problem. The organelles are complex 3‐D structures contained within cell bodies and the simple act of measuring the dimensions of the organelles can be extremely challenging. Traditionally, measurement of size would require laborious serial‐section electron microscopy (EM), followed by stereometric techniques to infer size descriptors such as volume and surface area based on the edges of the structure observed in individual sections. Use of electron tomography can simplify the task of measuring volume by directly acquiring the entire organelle, and the ability of tomography to be automated (Fung et al., 1996) is gradually helping this approach to become more routine. However, it is still quite diYcult, requiring substantial technical skills, and the thickness of sections that can be

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imaged puts a strong upper limit on the size of an individual organelle that can be imaged entirely in a single tomographic data set. The fact that organelles in general have complex 3‐D structures also creates a challenge for mathematical analysis—which number should one use to describe size? Surface area and volume are obvious measures, but other shape descriptors may also be necessary such as Gaussian curvature. We thus see that the inherent three dimensionality of most organelles makes the study of size control extremely challenging, both from a technical point of view and from a mathematical point of view. By focusing attention on a single dimension, length, the problem of organelle size control can be vastly simplified. Although length control has been studied in a variety of structures, including bacteriophage tails and sarcomere spacing (reviewed in Marshall, 2004), we feel that flagella and cilia represent a particularly tractable situation for studying the mechanisms of biological length control. Flagella present an elegant solution to this problem as they protrude from the cell, away from the cell body, and thus are easy to image and observe. They are significantly larger than bacteriophage tails or bacterial hooks, obviating the need for EM—indeed it is easy to measure flagellar lengths even in living cells using the very simplest of light microscopes. They are also very easy to describe as their size changes in only one dimension, length, making this the only dimension in which measurements must be made to observe diVerences in total organelle size. 3. Studying Length Control in Chlamydomonas—the Green Yeast This review focuses on studies of flagellar length control in the unicellular green alga Chlamydomonas, which is without question the most convenient model organism in which to study flagella. Chlamydomonas is sometimes referred to as green yeast because it has many of the same practical advantages for doing genetics as yeast, such as the ability to work with both haploid and diploid cells, tetrad analysis, growth as colonies on plates, and a rapid life cycle. However, unlike yeast, Chlamydomonas has flagella that are virtually indistinguishable from cilia and flagella in animal cells. This allows the powerful genetics of this organism to be brought to bear on questions of flagellar assembly and function, and for this reason most of what we know about flagellar assembly, including the polarity of assembly and the process of IFT, was first discovered in Chlamydomonas (see reviews by Dutcher, 1995; Silflow and Lefebvre, 2001). Consequently, there is a rich legacy of pre‐ existing mutants in Chlamydomonas, which aVect flagellar assembly and length. These include fla mutants, which cannot assemble flagella at the restrictive temperature (Adams et al., 1982), lf (long‐flagella) mutants, which have abnormally long flagella (Asleson and Lefebvre, 1998; Barsel et al., 1988; McVittie, 1972), and shf (short‐flagella) mutants, which have abnormally short flagella (Jarvik et al., 1984; Kuchka and Jarvik, 1987). Most of these mutants are

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available from the NSF‐sponsored Chlamydomonas Genetics Center stock collection. In addition to its genetic advantages, Chlamydomonas is also an excellent system for molecular biology, as it is easy to transform with DNA using simple methods (e.g., by electroporation), protein localization can be visualized using green fluorescent protein fusions, and gene expression profiles can be obtained using cDNA microarrays that have just become available. Completion of the Chlamydomonas genome, as well as establishment of a large database of EST sequences, has solidified this organism’s position as the premier model system for studying flagellar structure and function. B. Flagella and Cilia The terms flagella and cilia refer to essentially identical organelles, and we will use the two terms interchangeably. Historically, Chlamydomonas researchers have used the term flagella exclusively, so we will use this term in this review. However, we urge the reader to use the term cilia whenever possible, to avoid confusion with bacterial flagella, which bear no relation whatsoever to eukaryotic flagella. 1. Structure and Composition Flagella and cilia are microtubule‐based structures consisting of nine doublet microtubules nucleated by modified centrioles known as basal bodies. The microtubule doublets extend from the cell, and are surrounded by an extension of the plasma membrane. These doublets are all oriented with the microtubule plus‐ends located at the distal tip of the flagellum, and the minus‐ends located at the basal body located at the cell surface (Fig. 1). The term axoneme describes the microtubule doublets themselves along with the structural components that hold them together. Cilia and flagella are highly conserved throughout evolution, appearing in virtually identical forms in vertebrates, invertebrates, algae, lower plants, and protists. Although flagella and cilia are generally thought of as motile structures, many cells contain immotile cilia likely to play a sensory role (Marshall and Nonaka, 2006). For instance, a class of somatostatin receptors (Handel et al., 1999) is located on immotile cilia in the brain. Indeed, most sensory input to an animal is provided via sensory cilia, including both olfaction and vision (rods and cones being, in essence, highly modified cilia). 2. Human Diseases Involving Length Control Defects Given the near ubiquity of cilia and flagella in various tissues, it should not be surprising that many human diseases and their animal models appear to involve defects in cilia or flagella (Pazour and Rosenbaum, 2002). Examples include

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Nucleus = Dynein motor = Kinesin motor = Tubulin subunit = Lengthosome

? = IFT protein = LF4 protein = Disassembled tubulin subunit

FIG. 1 Diagram of flagellum showing components involved in length control. Intraflagellar transport (IFT) proteins capture flagellar protein precursors from the cytoplasm and transport them to the tip of the flagellum, the site of turnover. This movement is driven by kinesin‐II, and the retrograde movement of the IFT complexes back to the cytoplasm is driven by cytoplasmic dynein. IFT also transports the length‐regulating kinase LF4, although the function of this protein in the length control system is not yet fully understood. Three other length control proteins, LF1–LF3, localize within the cytoplasm in a structure called the lengthosome. This complex somehow regulates length, but its mechanism is not known. Genes encoding flagellar proteins are upregulated when flagellar regeneration is triggered by deflagellation, implying that some sort of signal reaches the nucleus, but the nature of this signal is not known. Thus, although many of the key players are identified, the systems level question of how they act together to produce a well‐defined length remains unanswered.

polycystic kidney disease (Haycraft et al., 2001; Pazour et al., 2000), biliary cystogenesis (Masyuk et al., 2003), male infertility (Chemes et al., 1990; Toyama et al., 1996), situs inversus, chronic sinusitis (Toskala et al., 1995), nephronophthisis (Otto et al., 2003), and Bardet‐Biedl syndrome (Ansley et al., 2003). In many cases, disease pathology involves the presence of abnormally short cilia or flagella (Chemes et al., 1990; Masyuk et al., 2003; Ortug, 2003; Pazour et al., 2000; Toskala et al., 1995; Toyama et al., 1996). This suggests that to understand, and possibly develop treatments for such diseases, we will need to understand not only what functions these cilia and flagella provide in human physiology, but also the mechanisms that specify their assembly and length determination. Because human cilia are highly homologous to Chlamydomonas flagella, both at the

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level of ultrastructure as well as in terms of their molecular composition, it is to be expected that lessons learned from flagellar length control will be directly applicable to the study of human ciliary disease. 3. Intraflagellar Transport and Flagellar Assembly Flagellar assembly is a particularly fascinating biosynthetic process because it occurs in a highly polarized manner (Johnson and Rosenbaum, 1992; Rosenbaum and Child, 1967). When flagella assemble, addition of new subunits (e.g., tubulin) occurs exclusively at the tip. In contrast, all protein synthesis occurs in the cell body, the flagellum being completely devoid of ribosomes. Therefore, flagellar precursor proteins must be transported to the distal tip of the flagellum where they are assembled. This transport is achieved by a process called intraflagellar transport (IFT, see Fig. 1) in which a pair of protein complexes (IFT complex A and IFT complex B) are moved from the cell body out to the tip by a kinesin motor and then returned to the cell body by cytoplasmic dynein (Cole, 2003; Scholey, 2003; Sloboda, 2002). The IFT protein complexes directly bind to flagellar precursor proteins in order to bring them to the tip (Qin et al., 2004, 2005). At the tip, the A and B subcomplexes undergo a rearrangement ultimately activating cytoplasmic dynein 1b, which then brings the IFT proteins back to the base of the flagellum (Pedersen et al., 2006). The process of IFT can be broken down into four distinct phases, that is, initiation of movement from the base, movement out to the tip, reversal of direction at the tip (accompanied by rearrangement of complexes), and then movement back to the base. These four phases can be measured in kymograph analyses, and it has been shown that mutants exist that diVerentially aVect various phases (Iomini et al., 2001). The molecules that regulate the switching between these phases remain unknown. Although IFT and its role in flagellar assembly were first discovered in the green alga Chlamydomonas, the process is highly conserved and involves the same set of molecules in all organisms that have cilia or flagella, including humans. Flagellar assembly at the tip not only occurs when the flagellum first grows, but also continues even after the flagellum has reached its final length (Marshall and Rosenbaum, 2001; Song and Dentler, 2001; Stephens, 1999). This steady‐state assembly is necessary to balance a continuous removal of subunits from the tip of the flagellum that occurs even once the flagellum has reached its final length. The continuous assembly and disassembly at the flagellar tip result in continuous turnover at a steady state. The teleological purpose of this turnover is unclear, but it may have first evolved as a mechanism to allow disassembly of cilia and flagella prior to cell division (Grimes and Gavin, 1987; Parker and Quarmby, 2003). Flagella are normally present in cells during the G1 growth phase and are resorbed prior to mitosis.

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Resorption can also be triggered by various chemical agents, and the mechanisms that mediate this resorption are currently the object of intense study (Pan and Snell, 2005; Parker and Quarmby, 2003), but one possibility is that it involves an upregulation of the underlying steady‐state turnover rate. The steady‐state assembly requires IFT to provide subunits for assembly (Adams et al., 1982; Piperno et al., 1996), and when IFT is turned oV in full‐length flagella, the flagellum immediately begins to resorb. Another interesting question is the mechanism of turnover. Flagellar axonemal microtubules are completely stable when isolated, suggesting they are not simply disassembling via conventional microtubule depolymerization. Instead, it appears tubulin turnover may involve exchange of tubulin at the junction between the two microtubules of the doublet (Stephens, 1999, 2000), via an unknown mechanism. It would be of great interest to identify the proteins that catalyze axonemal microtubule turnover, but so far there is no information about their identity. Given that the turnover occurs at the tip of the flagellum (Marshall and Rosenbaum, 2001), the disassembly machinery must be localized to the tip. It is known that the tip contains a morphologically distinct structure known as the ‘‘tip structure’’ (Dentler and Rosenbaum, 1977) but its composition or function is unclear. The microtubule plus‐end tracking protein EB1 also localizes to the tip (Pedersen et al., 2003), and this may play a role in regulating turnover, either directly or by recruiting other factors.

C. Phenomenological Studies of Flagellar Length Control 1. Measurement of Flagellar Length Distributions Because flagella are so easy to observe, there is a wealth of quantitative information concerning flagellar length variations under diVerent conditions. These experiments set the boundary conditions that any length control model must satisfy. Flagella are roughly 10‐ to 14‐microns long, although their average length depends on time of day and cell cycle progression (Tuxhorn et al., 1998). The fact that flagellar length is in a size range easy to measure using simple methods of light microscopy is one of the main reasons why this organelle is so useful as a model system to study size control. The first fact established by observations of flagella is that length appears to be under tight control. Specifically, measurements of the distribution of lengths in a population of Chlamydomonas cells appear to indicate length must be actively adjusted. What, exactly, does this statement mean? Careful measurements on synchronized cells (gametes, for instance) show flagellar lengths have an approximately Gaussian distribution with an average length around 10 microns and standard deviation in length of approximately 1 micron. Similar distributions of ciliary lengths are seen in other organisms

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(Wheatley and Bowser, 2000). The low coeYcient of variation of these length distributions provide a visual impression that length control is somehow ‘‘tight’’ in the sense that the variation in lengths is less than what we might expect in the absence of a control system. Why is this? Consider the length distribution that would be expected if there was NO length control. Suppose flagellar precursor subunits were assembled randomly into the flagella. What length distribution would result? Simple calculations show the length distribution for a simple single‐stranded linear equilibrium polymer should follow an exponential distribution, with the majority of the polymers having a short length (Nossal and Lecar, 1991). This would obviously not fit the Gaussian distribution seen in actual flagella. On the other hand, it is highly questionable whether a structure as complex as the flagellum should be considered a simple equilibrium polymer at all. Certainly a better approximation might be a multistranded dynamic polymer such as a microtubule, especially given experimental data that flagella are dynamic structures undergoing continuous turnover (Marshall and Rosenbaum, 2001; Stephens, 1999). Multistranded equilibrium polymers still show an exponential length distribution (Howard, 2001), as do dynamic polymers undergoing dynamic instability when confined within a cell, as judged by both experimental measurements and theoretical modeling (Dogterom and Leibler, 1993; Verde et al., 1992). If a dynamic polymer is allowed to grow without bounds, the length distribution can begin to approach a Gaussian (Verde et al., 1992), but theoretical models require such a distribution to have a constantly increasing average length over time (Verde et al., 1992). The fact that Chlamydomonas cells arrested in their growth cycle (e.g., gametes), can maintain a Gaussian distributed length with a constant average length, indicates that the length distribution cannot simply be accounted for by the same mechanism that functions in individual microtubules. To summarize this discussion, our naive visual impression that length is somehow restricted in its variation by a specific mechanism is likely to be correct. Two other important results are obtained from simple length measurements. First, although there is a certain degree of variability in lengths among a population of cells, the two flagella within a single cell are always more similar to each other than they are to the population in general. This suggests there might be an additional mechanism for equalizing lengths within one cell, above and beyond that involved in setting the length in the general population. It also suggests the dominant source of length variation in a population may be caused by cell–cell variation, as opposed to random temporal fluctuations within the activity of the length control system itself. Length variation is thus dominated by so‐called ‘‘extrinsic’’ noise (Elowitz et al., 2002). Second, flagellar lengths do not noticeably fluctuate in wild‐type cells during a normal observation period. Upon extended observation, it can be seen that lengths gradually increase over the course of a day. It would be

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interesting to know whether this is due to a simple increase in cell mass or biosynthetic capacity as the Chlamydomonas cell grows during the light phase, or whether instead this is due to a more direct influence of the cell cycle or circadian clock machinery on the length control system. Careful measurement of variation (i.e., noise) in flagellar lengths in Chlamydomonas cells grown under various conditions shows that there is a large reduction in the length variance when gametes are compared to asynchronously growing wild‐type cells (our unpublished data). Because gametes are arrested in a G0‐like stage of the cell cycle, this diVerence suggests variation in progression through the cell cycle is a major contributor to the extrinsic noise in flagellar length. Further evidence flagellar length is under specific control is obtained from other types of algal cells in which flagellar length varies reproducibly depending on the age of the basal body and cell cycle progression (Beech and Wetherbee, 1990; Lechtreck et al., 1997). Such results indicate flagellar length must be under active control, and the basal body is able to exert an influence in cis on its associated flagellum. 2. Flagellar Regeneration Much can be learned about a structure by watching how it is assembled. For most organelles, this is quite challenging because one cannot induce the organelle to form in a controlled fashion. Usually, the cell decides when it wants to build an organelle. One major advantage of flagella as a model system for organelle assembly is that one can, in Chlamydomonas, induce flagellar assembly in a highly defined and synchronous manner. This is because Chlamydomonas cells are able to sever their own flagella in response to a transient reduction in extracellular pH, a phenomenon known as flagellar autotomy. When cells are exposed to a pH shock, a complex signaling cascade is set in motion that ultimately leads to a katanin‐mediated severing of flagellar axonemal microtubules. The flagellum is then shed into the media, and a new flagellum begins to grow. The flagellum generally shows a lag of up to 10 min before growth begins, and growth typically reaches full length in less than 2 h. An alternative way to induce flagella to grow is to start with cells grown on a plate of agar media. For unknown reasons, Chlamydomonas cells grown on plates have flagella that are extremely short or even lacking entirely. Once the cells are washed oV into liquid media, they rapidly grow flagella reaching full length in less than half an hour. The first insight one gains from observing flagellar regeneration is that flagella do not grow at a uniform speed. Plots of growth curves show flagella grow at their maximum speed when they first start growing, and then continuously slow down, so that they asymptotically approach their final length. Most of the growth is over within the first hour. This type of kinetics has given rise to several diVerent interpretations. One interpretation is that

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the slowdown in growth shows that flagella grow under the control of a negative feedback loop such that the growth rate is highest when the length is maximally far from the desired set‐point, and then slows down as the set‐ point is reached. This interpretation seems unlikely to be true for the following reason. If cells are pretreated with cycloheximide, which blocks new protein synthesis, and then induced to shed their flagella, the new flagella that regenerate only grow to approximately half of the wild‐type length. Thus, they are far from their normal set‐point when they stop growing. Yet they show the same type of kinetics as normal flagella, with a rapid growth early on and a gradual approach to the final length over a roughly 1–2 hour period (Rosenbaum et al., 1969). If the growth rate were simply set by a feedback control that measured distance from the set‐point, then the slowdown in growth should only be observed when the flagella reach the set‐point length, which they never do in the cycloheximide experiment. A second possible explanation for the observed kinetics might be that the induction of flagellar assembly activates a defined intracellular signaling program, which directly determines growth rate as a function of time. This also seems unlikely because when cells with half‐length flagella, formed by regeneration in cycloheximide, are fused to wild‐type cells, the wild‐type cytoplasm allows the half‐length flagella to grow to the wild‐type length. When the growth kinetics in such experiments are compared to those in wild‐type flagellar regeneration, the growth rate at any given point in the elongation process correlates exactly with the length reached at the point, and not with the time elapsed since induction of growth (Marshall et al., 2005). The third interpretation is that growth rate is inherently length‐dependent due to a length‐dependence of intraflagellar transport. This possibility will be discussed in detail in the section on models for length control. Interestingly, when cells first form flagella, they do so with a dramatically diVerent type of kinetics. Madey and Melkonian (1990) measured flagellar outgrowth in Chlamydomonas cells after mitosis, before hatching from the mother cell wall would normally have occurred. They found in such cells, flagellar growth was completely linear, occurring at a constant, slow rate of 28 nm/min. This constant linear growth contrasts sharply with the decelerating growth seen during regeneration, and suggests a diVerent assembly mechanism might be at work. One possibility would be flagellar assembly at this stage might be strictly rate‐limited by a lack of a pre‐existing pool of precursor protein. In this case, the assembly rate is never able to become large enough for the length‐dependent eVects of IFT to become apparent. Consistent with this idea, Madey and Melkonian (1990) found that the postmitotic flagellar growth phase could be completely arrested by addition of cycloheximide. Thus, there are two types of flagellar assembly kinetics, apparently depending on the degree to which a cell has accumulated a precursor pool. The presence of these same two types of growth kinetics has also been reported in the closely

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related alga Volvox carteri (Coggin and Kochert, 1986) and is therefore probably a general phenomenon. It has been shown that flagellar growth in a related green alga, Spermatozopsis similis, occurs exclusively via an extremely slow linear kinetics (Schoppmeier and Lechtreck, 2003), suggesting that in this organism, unlike Chlamydomonas, IFT may either not be involved, or else be under dramatically diVerent regulation. At the very least, the fact that the flagella grow so slowly in Spermatozopsis (about 1 micron/h, compared to Chlamydomonas in which a flagellum can grow to 10 microns in 20 min) suggests the growth mechanism in Spermatozopsis occurs via a distinct process. Although this means results in this organism cannot be directly used to test the mechanism of length control in Chlamydomonas (Beech, 2003), it suggests a careful analysis of what is actually occurring in Spermatozopsis, using genetic and biochemical methods, might eventually provide some extremely useful insights into length control. The second insight resulting from studies of flagellar regeneration is that when flagella elongate, they do so by adding new protein exclusively at their distal ends (Johnson and Rosenbaum, 1992; Rosenbaum and Child, 1967). This conclusion, reached by pulse‐labeling cells undergoing elongation, would have been diYcult to obtain had it not been so easy to induce flagellar growth at the time of ones choosing. Similarly, studies of mRNA levels as a function of time after flagellar regeneration begins, have revealed cells execute a complex program of transcriptional activation, with several hundred genes upregulated (Lefebvre et al., 1980; Stolc et al., 2005) leading to concomitant increases in protein levels of flagellar precursor proteins (Lefebvre et al., 1978). Interestingly, when Chlamydomonas flagella are induced to elongate by addition of the drug lithium, this elongation also triggers induction of flagellar genes (Pena, 2005). Although the molecular pathway that regulates this gene induction program is unknown, mutants have been identified in which induction no longer occurs (Lefebvre et al., 1988). It will be extremely interesting to learn the precise nature of the pathway that drives flagellar gene expression. Because most current methods used to study gene expression are based on analysis of whole populations of cells, the ability to induce synchronous flagellar regeneration in a whole population of Chlamydomonas cells has been invaluable for these studies. The role of this transcriptional program in length control remain unclear, given that cells in which protein synthesis is blocked are still able to reach a defined length, albeit one that is shorter than normal. 3. Flagellar Length Equalization One of the most dramatic phenomena pertaining to flagellar length control is the equalization of flagellar lengths following a transient perturbation. This is observed experimentally by removing one of the two flagella from a cell,

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and then observing the behavior in real time. Technically, the challenge to this experiment is how to remove just one of the two flagella. In some organisms with very large flagella, this can be done by direct micromanipulation (Tamm, 1967). In Chlamydomonas, this has been accomplished by blending a suspension of cells in a Waring blender. If the shear forces are adjusted properly, a significant fraction of the cells will shear oV just one flagellum. After shearing, cells are examined under a microscope, and once a cell is found that has only one flagellum, it can be tracked over time to observe the behavior. The behavior of cells from which one flagellum has been removed is quite remarkable, and has had a major impact on our conceptual view of flagellar length control as an active process. In such cells, the severed flagellum begins to regenerate, following similar kinetics to those seen in flagellar regeneration as previously described. However, while this growth is occurring, the other flagellum begins to shorten! The long flagellum continues to shorten while the regenerating flagellum grows, until they reach the same length. At that point, the two flagella grow out together. If cells are treated with cycloheximide, to poison new protein synthesis, then the two flagella will converge on the same length but will not undergo further growth. In some cases, the long flagellum overshoots the short flagellum transiently, but in such cases it eventually returns to the same length. This ability of cells to equalize the lengths of their flagella has been taken to indicate the long flagellum somehow ‘‘knows’’ it is too long, or it is ‘‘instructed’’ by the cell to shorten. To some extent, this view was a byproduct of a mistaken idea of flagellar stability. Before studies of flagellar protein turnover were performed (Marshall and Rosenbaum, 2001; Stephens, 1999), it was generally assumed flagellar microtubules were perfectly stable (Tilney and Gibbins, 1968). This was thought to be the case because flagella do not disassemble when isolated in vitro, nor do they shorten when microtubule depolymerizing drugs are applied. If flagella are in fact stable, then the length equalization process would necessarily entail an activation of some disassembly machinery. However such a disassembly would not, or so the reasoning went, be active in the regenerating flagellum, or else it would not be able to grow. For this machinery to be activated in the long flagellum, but not in the short one, there must be a regulatory pathway diVerentially activated in the long versus the short flagellum. In other words, the long flagellum must know it is too long. However this argument is based entirely on the mistaken view that flagella are static structures. The fact that flagella are dynamic structures, undergoing continual turnover, provides an alternative explanation for the length equalization. In a cell with two flagella, these two flagella are competing for a common pool of precursor protein. During flagellar regeneration, flagella grow extremely quickly when they are short, and grow with a decelerating kinetics such that their growth rate decreases as length increases. Because turnover continues even after flagella reach full length, the assembly rate

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never quite becomes zero, but attains some small finite value to balance the ongoing removal during turnover. If one flagellum is suddenly shortened, it will grow with a much faster assembly rate than the full‐length flagellum. Because when a flagellum grows, it incorporates precursor protein from the cytoplasmic pool, the rapid growth of the regenerating flagellum will necessarily choke oV the supply of precursor from the longer flagellum. In essence, the short flagellum will be able to take more than its fair share of the cytoplasmic protein pool. This will then cause the assembly rate in the long flagellum to decrease to the point that it no longer balances disassembly during turnover, and as a result the flagellum will begin to shorten. The disparity in assembly rates will hold as long as the two flagella are of unequal length. Numerical simulations have shown that this type of mechanism can account for the length equalization seen in experiments (Marshall and Rosenbaum, 2001). Therefore, it can no longer be claimed that flagella know how long they are, in the sense of having regulatory pathways whose activity depends on length, simply on the basis of the flagellar length equalization experiments. Another example of flagellar length equalization has been reported using mutant cells having recessive mutation that cause their flagella to be longer than wild‐type. These mutants are discussed in detail in Section D. When these long flagella cells are fused to wild‐type cells, it has been observed that the abnormally long flagella shorten until they reach the same length as the original wild‐type flagella from the wild‐type cell. In this case the length equalization is simply due to the fact that the mutations causing the abnormally long flagellar length are recessive, so that when mixed with wild‐type cytoplasm, the recessive mutation is rescued and the length reverts to normal. This experiment, therefore, tells us something about the nature of the mutations, but certainly does not constitute evidence for an active length‐change– inducing regulatory pathway within flagella. As with the length equalization experiments discussed in the preceding paragraph, the length equalization response in cell fusion experiments with long‐flagella mutant cells has also been recapitulated using numerical simulations that rely only on turnover and do not invoke any specific signaling pathway (Marshall and Rosenbaum, 2001). To summarize this section, we can say that flagellar length equalization is now understood to reflect that flagella are dynamic structures, undergoing continual turnover, and that their assembly rate depends on length.

D. Genetic Analysis of Flagellar Length Control Whenever attempting to learn about a new biological system, one way to shine light into the ‘‘black box’’ is genetics. Genetic screens in Chlamydomonas have revealed a set of genes aVecting flagellar length control.

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1. Identifying Length Mutants in Chlamydomonas Genetic Screens Because flagella drive Chlamydomonas cell motility, flagellar length defects can be isolated in motility screens. The general procedure is to mutagenize cells, pick individual colonies into tubes or microwells, and then examine cell movements under a dissecting microscope. This method has been used to identify both short‐flagella mutants (Kuchka and Jarvik, 1987) and long‐ flagella mutants (Asleson and Lefebvre, 1998; Jarvik et al., 1976, 1980; McVittie, 1972). Because this screening strategy requires each mutagenized colony to be individually examined by a human observer using a microscope, it is exceedingly tedious and diYcult to perform on a large scale. Thus it seems likely the screens conducted to date are far from saturation, and many more long‐ and short‐flagella mutants could be obtained if screening methods with higher throughput could be devised. The diYculty of identifying long‐flagella mutants by visual genetic screens has therefore prompted a search for more eYcient strategies. In a very clever approach, Lefebvre’s group noticed many long‐flagella mutants also show reduced rates of flagellar regeneration after pH‐induced flagellar autotomy. Based on this observation, they reasoned that long‐flagella mutants could be enriched by first screening for mutants defective in flagellar regeneration, followed by a secondary visual screen for length alteration. Using this approach, coupled with a high‐throughput screen for flagellar regeneration mutants, they were able to identify long‐flagella alleles of a new gene, LF3 (Barsel et al., 1988). We note, however, that not all long‐flagella mutants show such a delay in flagellar regeneration, indicating that a screen based on this criterion will not be able to identify all potential long‐flagella mutants, but only those that have this additional phenotype. Therefore, a need still exists for a rapid and scalable screening method based on automated measurement of either flagellar length directly or of motility.

2. Phenotypic and Genetic Analysis of Long‐Flagella Mutants It is also important to consider phenotypes other than an overall increase or decrease in length. Indeed, if one considers that length is maintained by a control system, if the system were to be truly broken by a mutation, then one might expect that the predominant phenotype would be failure to maintain a unique consistent length. If a mutation causes all cells to shift to a new, longer length, this indicates that the length control system is still functioning, but has simply been reset to a new set‐point. Such mutations would therefore reveal genes involved in setting the control point of the system, but not in the functioning of the system itself. Thus, the most interesting mutants would be those resulting in a randomization or increased fluctuation in length from cell to cell.

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In fact, such mutations have been found, and interestingly, they appear to represent alleles of previously identified length genes. The original lf2 and lf3 alleles were all induced by chemical mutagenesis or UV and may not have resulted in null alleles. It turns out null mutations in the LF2 and LF3 genes result in a phenotype in which the average flagellar length is not particularly long. Instead, the main defect observed is that the flagellar lengths within a given cell are unequal, a phenotype known as unequal flagellar length (ULF). This was discovered in insertional mutagenesis screens for mutations that gave the ulf phenotype. Two ulf mutants identified in this screen, ulf1 and ulf3, were found by genetic analysis to be alleles of LF3 (Tam et al., 2003). These mutant cells mostly lacked flagella, and when flagella were present, they were of unequal lengths and, interestingly, shorter than the average wild‐type length. It may at first seem puzzling or paradoxical that null alleles of a long‐flagella gene have abnormally short flagella, but bear in mind that the main phenotype of lf1, lf2, and lf3 mutants is the increased variability in length—the average length is actually not that much more than wild‐type, and in a population of lf mutant cells, many flagella are quite short while others have unusually long flagella. This is true even in many original lf alleles. These results imply that the LF genes are aVecting flagellar dynamics in a subtle way. 3. Intraflagellar Transport in Length Mutants Given that intraflagellar transport is required to maintain flagellar length, it is obvious to ask whether any length mutants aVect the process of IFT. Certainly, partial reductions in IFT do in fact result in shorter flagella, for instance fla2 mutant cells, which have a reduced velocity of IFT particle motion at the permissive temperature (Iomini et al., 2001) have flagella that are significantly shorter than wild‐type (our unpublished observations). What about long‐flagella mutants? In this case the evidence is much less clear, but IFT is so obviously a candidate for involvement in length control, that it makes sense to check whether known lf mutants might increase the rate of IFT. To some extent, this is like a drunk looking for his keys under the street lamp for the sole reason that this is where the light is brightest. Because we know more about IFT than we do about most aspects of flagellar assembly, it makes a good starting point for analyzing the eVects of lf mutations. In any case, detailed information about how distinct alleles of the lf genes aVect transport and turnover within the flagellum is likely to yield new insights into the length control machinery. It has been demonstrated that flagella in LF3 null mutants show an increase in the quantity of IFT proteins relative to wild‐type (Tam et al., 2003). This result seems at first glance to explain the lf3 mutant phenotype: lf3 mutant flagella have increased IFT, allowing them to grow more rapidly

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to a longer final length. Unfortunately, this cannot be the whole story because the increased IFT protein levels were measured in an insertional allele of LF3 (lf3–5) in which flagella are actually shorter on average than wild‐type. If increased IFT protein leads to a longer flagellum, why are the lf3–5 flagella shorter? In actuality, the apparent increase in IFT proteins in lf3 mutants is potentially misleading. It has previously been shown, both by immunofluorescence and Western blotting (Marshall and Rosenbaum, 2001; Marshall et al., 2005) that the quantity of IFT protein within the flagellum is independent of length, such that very short flagella contain the same total quantity of IFT protein as very long flagella. Consequently, in cells with short flagella such as those seen in lf3–5, the IFT proteins will always represent a disproportionate fraction of the total protein simply because their quantity per flagellum remains constant regardless of length whereas the total axonemal protein content per flagellum is reduced in shorter flagella, so that if Western blots are run loading the same total protein, as was done by Tam et al. (2003), one would expect any short flagella will show an increase in IFT. Therefore, the increased fraction of total protein represented by IFT proteins in the LF3 null mutant does NOT indicate that the LF3 gene product regulates IFT. Quite the contrary, this result suggests IFT levels are normal in the LF3 null mutant. It thus remains unclear how the lf3 mutation aVects length. An interesting clue comes from extensive ultrastructural analysis of lf3 which revealed linear aggregates of material accumulating at the tips of the short flagella, like a bag full of toothpicks. Although the authors who conducted the study interpreted this material as IFT protein aggregates, it is equally possible that these linear structures represent defective assembly of axonemal components, suggesting a role for LF3 in regulation of assembly. 4. Length Control Proteins—Localization and Function In addition to serving as tools to probe the behavior of the length control system, length mutants also allow us to identify the protein components of the system itself, once the genes are cloned. A major ongoing eVort by the Lefebvre laboratory has resulted in the identification of all four LF genes. Both LF1 and LF3 are apparently novel genes (Nguyen et al., 2005; Tam et al., 2003). However, identification of the genes provides a foot in the door. For instance, epitope tagging has led to new and interesting information about subcellular localization. Both LF1 and LF3 appear to localize in the cell body rather than the flagellum, and both localize in a number of punctate foci. This suggests that LF1 and LF3, and possibly other length control proteins, colocalize together in a cytoplasmic substructure which has been dubbed the ‘‘lengthosome’’ (see Fig. 1). How the activity of the lengthosome functions to regulate flagellar length remains unknown.

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LF4 was found to encode a protein kinase of the MAP kinase family (Berman et al., 2003). LF4p localizes both to the cytoplasm and also within the flagellum and is apparently regulated by a phosphatase located within the flagellum (Wilson and Lefebvre, 2005). The fact that LF4 is a kinase indicates a signal transduction pathway is involved in length control. It is tempting to speculate that this might represent a feedback control pathway, in which a length sensor reads flagellar length, modifies the activity LF4 accordingly, and then LF4 signals to a downstream pathway that adjusts length. There is, however, no evidence so far that LF4 actually functions within a feedback loop. It is just as likely, a priori, that LF4 acts in an input pathway to the length control system, by which the cell can specify how long the flagella ought to be. The only evidence in favor of a feedback function, so far, is the presence of LF4 protein within the flagellum. This might seem hard to reconcile with a purely input‐pathway function for LF4, unless LF4 has to carry its signal to the flagellar tip, for example, to provide its input to the pathway. It is clear further investigation of LF4 will be of great interest. To summarize the genetic analyses of flagellar length control, four long‐ flagella genes have been cloned, LF1 through LF4, of which LF1–LF3 appear to localize together in cytoplasmic ‘‘lengthosome’’ complexes of unknown function, whereas LF4 is a MAP kinase that can be found within the flagellum. These genes provide a starting point to dissect the molecular pathway of length control. They also provide invaluable tools for testing potential models for the length‐control mechanism.

III. Models for Flagellar Length Control System Given the extensive set of genetic and phenomenological data that exist concerning flagellar length control in Chlamydomonas, this system represents a best‐case situation for developing and testing mechanistic models for length control. In this section we consider five broad classes of theoretical length‐ control mechanisms that have been suggested to account for length control in various cellular systems (Marshall, 2004). We will consider which of these may be applicable to the specific problem of flagellar length control in Chlamydomonas. A. Molecular Ruler One mechanism used in length control is a molecular rule, in which a protein molecule is produced whose physical length matches the length of the structures whose size is to be controlled. One end of the ruler molecule is anchored at the point where the polymeric structure begins its self‐assembly, and then

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the other end tracks the growing end of the polymeric structure, either promoting assembly directly or acting as a protective cap to block access of the growing end to diVusible growth‐inhibiting factors. This type of mechanism is clearly at work in the case of bacteriophage tail fibers (Katsura, 1990) and is also implicated in the control of actin filament length within striated muscles (Fowler et al., 2006). The key prediction of a molecular ruler model is that a protein must be identified whose length matches the assembling structure. Such a protein has not yet been identified for the flagellum, although we must admit failure to discover something hardly constitutes proof of its nonexistence. In general, though, molecular rulers tend to be employed for size control in small structures less than a micron long, which makes sense given that the size has to be set by a single protein, and there is a limit to how long a protein can be. Again, though, we do not strictly know what this limit is. Moreover, there are ways to get around the need for a single long protein— one can theorize vernier‐type mechanisms where a pair of proteins of slightly diVerent length assemble alongside one another and only when their two ends line up flush with each other can they recruit a factor to define the assembly termination point. In this case, the length is set by the least common multiple of the lengths of the individual elements. In such a vernier system, it might be very hard to know a priori that a given protein is part of the vernier system, because it would assemble alongside the axoneme and to all intents and purposes be part of it. Because the component proteins of a vernier ruler would not have to be particularly long, there is no obvious feature that would reveal them to us. Is there any conceivable way to rule out a ruler model then, given that we cannot rest on the absence of direct demonstration of the ruler itself? One approach is theoretical, as described by mathematical analyses of the ruler mechanism (Wagenknecht and Bloomfield, 1975); the distribution of lengths produced by a ruler shows a very skewed distribution. Conceptually this can be understood because a protein has a certain degree of flexibility, hence the ruler protein can sometimes flex to a shorter end‐to‐end length, allowing structures of a reduced length to form with some probability. There is a hard cut‐oV at longer lengths, however, because there is a limit to how far the ruler can stretch. This leads to a distribution skewed to shorter lengths. Our own measurements (W. Marshall, unpublished data) show flagellar length distributions in wild‐ type Chlamydomonas cells show an essentially Gaussian distribution, based on statistical calculations of skew and kurtosis. This would seem to rule out ruler models of the simplest type based on a single long flexible ruler protein. However, for a vernier system that coassembles alongside the highly rigid axoneme, it is unlikely that shorter structures can be produced. Moreover, if the ruler acts by interacting with a diVusible eVector, it might simply set the mean value of a Gaussian distribution of sizes whose variance is determined by the diVusion constant of the diVusing eVector. It is thus not possible to completely rule out a ruler model by this type of measurement.

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A better argument against rulers is the fact that in a population of cells, flagellar lengths can vary by 1–2 microns. Moreover, even in a single cell, the length varies during the course of the day. Length is also reduced when cells regenerate in the absence of protein synthesis as discussed earlier in the chapter. It is quite hard to reconcile these results with a single fixed‐ruler mechanism. One would have to propose that a ruler or vernier undergoes changes from cell to cell, throughout the day, and in response to changes in protein levels. While a suitably baroque model could probably be devised to incorporate all of these eVects, Occam’s razor suggests our time is better spent evaluating alternative length control methods.

B. Quantal Production The second type of mechanism we consider is the quantal production of limiting precursor. In this model, there is one (or possibly more) key structural protein constituent of the flagellum whose quantity is limiting. When a cell initiates formation of a flagellum, a certain quantity of this precursor is synthesized, and then it is incorporated into the growing flagellum. In this model, flagellar growth ceases when the quantity of this limiting precursor is exhausted. Supporting evidence for this type of model comes from experiments in sea urchin cells (Norrander et al., 1995; Stephens, 1989) in which the level of tektin synthesis was found to correlate with the length of cilia in various cells. However, correlation does not prove causality and from this data alone it would be equally plausible that protein production is sensitive to the length or growth of the flagellum. Direct evidence against the limiting precursor model comes from experiments in Chlamydomonas in which cells regenerate flagella in the presence of cycloheximide. In such experiments, flagella do in fact regenerate, albeit to approximately half the normal length. This demonstrates that even after flagellar assembly is completed, the cytoplasm retains a suYcient quantity of all precursor proteins to produce two half‐length flagella. Therefore, there cannot be a limiting precursor whose consumption sets the final flagellar length. Further evidence against the quantal production of limiting precursor model comes from experiments with Chlamydomonas mutants having variable numbers of flagella (Kuchka and Jarvik, 1982). Such mutants are called vfl, which stands for ‘‘variable flagella.’’ In the Kuchka and Jarvik study (1982), vfl2 mutant cells having a variable flagellar number between 1 and 4 were examined. If cells produced a fixed limiting quantity of a key precursor that was completely consumed during the process of flagellar growth, then the combined lengths of all flagella in a single cell must add up to the length of a flagellum that could be constructed from this limiting precursor quantity

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in a cell with a single flagellum. Hence, cells with two flagella should have flagella half as long as cells with a single flagellum. Flagella would be one third as long in cells with three flagella, and one quarter as long in cells with four flagella. This geometric dependence of length on flagellar number was not, however, observed. Instead, the lengths of the flagella decreased only slightly as their copy number increased. More extensive measurements on three diVerent vfl mutants (vfl1, vfl2, and vfl3), including measurements under diVerent fixation conditions and in living cells, have confirmed that the dependence of flagellar length on number does not match the geometric dependence predicted by the limiting precursor model (Marshall et al., 2005). Finally, one can ask whether a limiting precursor model can account for altered lengths in shf or lf mutants. In the context of this model, an lf mutant would increase length by generating increased levels of precursor protein. Such an increase has not been detected by Western blot analysis with known flagellar proteins. It could be argued that one might only see a major increase in protein quantity in those particular cells that make long flagella within a mixed population of lf cells showing a high variance in length, some short, some long. Because standard biochemical analyses are population‐based, they could not detect such a phenomenon at the level of the single cell and might fail to see a significant diVerence at the population level. We can, however, rule out this possibility by another experiment. If an lf mutant makes a drastically larger quantity of a key precursor protein, then if such cells were fused to wild‐type cells, the increased precursor levels in the combined cytoplasm should result in a cell with four longer‐than‐normal flagella. In fact, when lf mutants and wild‐type are fused, the two long flagella rapidly revert to wild‐type length (Barsel et al., 1988). This argues against the idea of a dramatically increased level of a specific precursor protein in such mutants, even if the increase is only seen in a few individual cells. It thus appears the quantal precursor model is not compatible with the observed genetic and phenomenological data.

C. Cumulated Strain Model A model has been proposed for bacteriophage tail length control, which theorizes that as additional subunits polymerize onto the growing structure, they undergo an increasingly great conformation alteration, such that the free energy of binding is gradually reduced by a constant increment (Kellenberger, 1972). This model, known as the ‘‘cumulated strain model,’’ has been investigated mathematically by Wagenknecht and Bloomfield (1975), who demonstrate that it can lead to an extremely tight distribution around some defined length, using biologically realistic parameters. Their model indicates that for a given precision of length control, the free energy change needed to explain that

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control becomes less and less as the number of subunits increases. Their model can account for length control in a phage tail with fewer than 100 subunits without invoking an unreasonable change in binding energy. Therefore, the change in energetics needed to fit length control in flagella, which contain tens or hundreds of thousands of subunits (depending on whether one considers a subunit a tubulin dimer or a whole 96‐nm repeating unit of axonemal structure) will be even less, and therefore certainly within a physically possible realm. The cumulated strain model is thus capable, in theory, of producing the degree of length regulation (in terms of the standard deviation of the length) observed in real flagella, at least in the sense that the change in free energy of binding that would have to be invoked will be extremely small. So, the model will not violate the laws of physics, which is of course important. But a somewhat more stringent test is to ask whether this model can account for all phenomenological and genetic data discussed in Sections II.C and II.D. The cumulated strain model predicts that if the ratio between the total quantity of monomer and the number of initiation sites (basal bodies, in our case) is altered, the length should change in defined ways (Wagenknecht and Bloomfield, 1975). Specifically, when the ratio drops, the length should decrease in proportion to the change in the ratio. This predicts cells with two basal bodies should have flagella twice as long as those with four, a prediction that is not borne out by experiments with vfl mutants (Kuchka and Jarvik, 1982; Marshall et al., 2005). Thus, this model fails the same test that excluded the quantal production model. We can also consider whether the cumulated strain model can account for the known shf and lf mutants. The only parameters that can really be changed in the model are the free energy change during successive polymerization steps, and the total quantity of monomer present. Therefore, if a length mutant is to result in altered length, it must change one or the other of these quantities. It is not obvious how proteins such as lf3, whose products localize to the cell body and are not components of the flagellum itself, could alter the binding energy of flagellar protein subunits. This leaves the alternative, that the lf and shf mutants alter the quantity of one or more key flagellar protein subunits. An interesting result of the analysis of the cumulated strain model, as shown by Wagenknecht and Bloomfield, is that although reductions in monomer quantity lead to proportional reductions in length, increases do not. The cumulated strain model is highly resistant to length increases beyond the normal length, such that to generate a detectable increase in average length, concentrations of monomer must be increased by several orders of magnitude. Such increases are simply not seen in lf mutants for flagellar proteins in general—for instance, tubulin does not appear to be made in significantly larger quantities in lf mutants. Strictly speaking, however, it is possible one or more unknown proteins are playing a key role in limiting length, and without a specific antibody to detect them, we might have no way of knowing whether they are suddenly produced in much greater

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quantities in an lf mutant. But as with the quantal precursor model, the fact that lf mutant cells with long flagella undergo rapid flagellar shortening to wild‐type length when fused with wild‐type cells, strongly suggests they do not contain elevated precursor levels. Therefore, it seems diYcult to make the cumulated strain model work out in the context of long‐flagella mutants. Overall, the cumulated strain model is diYcult to reconcile with specific experimental details of flagellar length control, at least in its simplest form. Whether a more generalized version of the model, perhaps with a diVerent dependence of binding energy as a function of polymerization extent, could overcome these problems, remains to be seriously explored.

D. Feedback Model A fourth type of length control system one could envision is a feedback control system. In this mechanism, a signal transduction pathway somehow senses the length of the flagellum, and then acts to modulate the assembly process to attain the correct length. For instance, a length‐sensing pathway could inhibit IFT when the flagellum is too long, or upregulate IFT when the flagellum is too short. For such a system to produce a flagellum of a defined length, the feedback would have to be negative. Thus, a length‐sensing pathway, if it acted upon IFT, would have to inhibit IFT as length increases. Feedback control systems are common in man‐made devices, and are known to confer desirable properties of stability and robustness. Feedback control requires a length sensor to provide the initial input into a signal transduction cascade that ultimately impinges on flagellar assembly machinery. How might length be sensed by a molecular mechanism? One proposal (Rosenbaum, 2003) is that flagella may contain a length‐dependent number of calcium channels, so that the total calcium current through the flagellar membrane would be length dependent. How calcium fluxes might lead to changes in flagellar length is unclear but could involve one or more of the known calcium‐dependent phosphorylation events that occur within flagella (Bloodgood, 1992). This model is consistent with measurements showing that the number of calcium channels in the flagellar membrane of Chlamydomonas is proportional to flagellar length (Beck and Uhl, 1994). However, as with the studies of tektin levels, correlation does not prove causality, and so it is just as likely that length aVects channel number rather than vice versa. An alternative model for measuring length would be to attach a molecular timer, such as a G‐protein, to the IFT complexes, load it with GTP using a GEF at the basal body region, and then check the nucleotide state of the G‐protein upon the return of the IFT complex from the flagellum. If the round‐trip time for a wild‐type length flagellum is comparable to the GTPase rate of the G‐protein, then deviations in length would result

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in measurable changes in the GTP/GDP ratio which could in turn modulate the activity of a length‐sensitive signal transduction cascade. Many other such models can be easily proposed, but the problem is finding a way to test them. Ultimately, the only way to determine whether a feedback control loop is involved in length control is to identify the potential signaling pathway and then test whether it is activated in a manner consistent with overall negative feedback. The most likely candidate for a length‐responsive signaling molecule is the LF4 kinase (Berman et al., 2003). As discussed earlier, lf4 mutants have abnormally long flagella. The mere fact that a kinase like LF4 results in a length change when mutated, does not by any means prove it is part of a feedback loop. For example, one could speculate the LF4 kinase might instead be present to allow the cell to alter the length of its flagellum in response to various environmental or developmental cues. The feedback control model does, however, make some simple predictions about LF4 that can be tested. Loss‐of‐function mutations in LF4 lead to increased flagellar length, hence the normal function of LF4 must be to oppose net flagellar assembly. Therefore, for this molecule to act in a negative feedback loop, its own activity must be an increasing function of flagellar length. In other words, LF4 kinase must be activated when flagella are too long, and inactivated when flagella are too short. It is thus conceptually straightforward to test whether LF4 is part of a length‐sensing feedback loop—one has only to measure the activation state of LF4 as a function of flagellar length. However, this measurement has not yet been reported. If the activity of LF4 is not in fact length‐dependent, then it cannot be acting in a feedback loop. Other possible signaling molecules involved in length control have been revealed by pharmacological studies (Wilson and Lefebvre, 2004). However the same caveats apply to these studies as to LF4—the detection of a signaling molecule does not prove it acts in a feedback pathway. To support such a claim, the pharmacological drug targets must be definitively identified (not a simple task in most cases) and then the activation state of these targets measured as a function of flagellar length and compared to the behavior required by the negative‐feedback constraint. Nevertheless, the identification of signaling molecules that impinge upon length control, primarily due to the groundbreaking work of Wilson and Lefebvre, is a major step forward because it leads to readily testable hypotheses about the molecular mechanism of length control.

E. Balance Point Model A simple model for length control has been proposed that does not require an explicit length sensor or signaling pathway (as in the feedback model). This model is based on the observation in Chlamydomonas showing axonemal microtubules undergo continuous turnover at their distal tip, and this turnover is balanced by new assembly, which in turn requires intraflagellar

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transport (Marshall and Rosenbaum, 2001). The rate of disassembly at the tip appears to be independent of length. Further analysis of IFT particles revealed the number of IFT particles per flagellum is independent of length (Marshall and Rosenbaum, 2001; Marshall et al., 2005). If a fixed number of transport particles are forced to move over a greater and greater length, the rate at which they can drop oV cargo to the tip and return for another load will decrease. Eventually, when the flagellum gets long enough, transport will no longer be eYcient enough to balance disassembly, and the flagellum will have to shorten. It has previously been remarked that the deceleratory kinetics of flagellar regrowth in Chlamydomonas require a reduction in IFT as elongation progresses (Beech, 2003). In our model, this reduction occurs via simple physics—when a fixed number of IFT complexes, traveling at a fixed velocity, then it takes them longer and longer to complete a transport cycle as the flagellum elongates. No special signaling or regulation is required apart from the obvious fact it takes longer for a moving object to travel a greater distance. The model as formulated is a macroscopic model, phrased in terms of lengths and rates. A more detailed microscopic model that describes the behavior of individual molecular components, has been evaluated and shown capable of producing a stable steady‐steady state length (BressloV, 2006), confirming the balance point model is at least theoretically reasonable. This model predicts that the flagellum will reach a unique length defined by a balance‐point between length‐independent disassembly and length‐ dependent assembly. This model can account for many observed aspects of length control, for instance the dependence of flagellar length on number in vfl mutants, the growth kinetics upon resumption of growth in half‐length flagella, the ability of flagella to equalize their lengths when one flagellum on a biflagellate cell is severed, and the shortening kinetics of long‐flagella mutant cells when fused to wild‐type cells (Marshall, 2005; Marshall and Rosenbaum, 2001). For two of these experiments, previous publications had presented data that appeared to be inconsistent with the balance‐point model. A previous study (Kuchka and Jarvik, 1982) reported flagellar length does not depend on number, however the data reported in that paper actually show just the opposite and confirm a report (Marshall et al., 2005) that cells with more than two flagella have a reduced flagellar length. Kuchka and Jarvik’s data suggested cells with one flagellum and cells with two flagella had equal lengths, but additional data suggests this is not generally the case (Marshall et al., 2005). A previous study suggested that when flagella arrested at half‐length resume growth by restoration of wild‐type gene function to a shf mutant, that these flagella initially grow with the same rate as a wild‐type flagellum growing starting at zero length (Jarvik et al., 1984). This suggests that growth rate is a function of time after growth induction, and not a function of length as predicted by the balance‐point model. However, re‐examination of the published data suggested an erroneous value for

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wild‐type growth rates, and when these experiments were repeated in two diVerent ways, in all cases the results support the model that growth rate depends strictly on length (Marshall et al., 2005). Thus, we conclude that the balance point model is compatible with all known phenomenological experiments on flagellar length regulation. The balance point model also accounts for the possibility of shf and lf mutants. In this model, shf mutants can arise in either of two ways: either the rate of turnover is increased, or the rate of transport is decreased. Confirmation of this latter possibility has been obtained by creating a partial reduction in IFT. This partial IFT reduction was achieved by growing temperature‐sensitive fla10 mutants cells, carrying a conditional mutation in the fla10 kinesin that drives IFT, at a temperature intermediate between fully permissive and fully nonpermissive. It was confirmed by western blot analysis that such flagella contain a reduced quantity of IFT protein (Marshall et al., 2005). This reduction in IFT was observed to produce a stable, persistent shift in length to a new length roughly half that of wild‐type cells (Marshall and Rosenbaum, 2001). This directly demonstrates that the shf phenotype can be obtained by reduction in intraflagellar transport, which is a prediction of the balance point model but NOT of any of the other models. We especially note that feedback control systems, when present, are able to maintain a stable set‐point even when the underlying process is perturbed (e.g., a thermostat can maintain room temperature even if the radiator is partially blocked by furniture, because it will lead to increased furnace activity to compensate). The fact that reduction in IFT levels leads to a decreased length is thus compatible with the balance point model but not the feedback control model. The lf phenotype can also be explained by the balance point model. Again there are two possibilities: a long flagellum can be generated either by a reduction in the rate of turnover or an increase in intraflagellar transport. The first possibility is potentially the case for lf2 mutants based on experimental measurements of tubulin dynamics in such mutants having shown them to have a reduced rate of turnover at steady state (Marshall and Rosenbaum, 2001). Similarly, the NIMA kinase Cnk2 exerts an influence on flagellar length apparently, at least in part, by modulating the disassembly rate (Bradley and Quarmby, 2005). In contrast, the long‐flagella mutant lf4 does not appear to alter its rate of turnover compared to wild‐type (Song and Dentler, 2001) suggesting lf4 flagella are long for some other reason. This model therefore seems capable of explaining all known experimental data concerning flagellar length control. However, the model faces one serious problem. The balance point model of length control requires the number of IFT particles active in the cilium be held constant. This prediction raises two questions: first, is it actually the case that the number of IFT proteins is constant, and second, by what possible mechanism could this constant quantity be achieved? Direct measurements, including both biochemical analysis of protein levels on Western blots (Marshall et al., 2005),

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quantitative measurements of immunofluorescence intensity (Marshall and Rosenbaum, 2001), and counting of IFT particles by immunofluorescence microscopy (Marshall et al., 2005), all show the quantity of IFT protein complexes within the flagellum is independent of length. Particle counting analysis indicates the number of particle aggregates is roughly eight on average, with a range of between seven and nine from cell to cell. How can an organelle count the number of particles within it? Kymograph data suggests a remarkably simple model for particle counting. As indicated in Fig. 2B, William Dentler (Dentler, 2005) has shown beautiful kymographs of IFT particle aggregates moving up and down within the flagellum in Chlamydomonas. His images strongly suggest that individual IFT particle aggregates move up and down within the flagellum without leaving it, because all of the kymograph traces of a particle moving upwards begin at the end of a trace of a particle moving downwards. Traces indicative of new particles being injected into the flagellum, which would not originate at the end of a downwards trace, were not observed in his images. These considerations suggest IFT might resemble a subway, in which passengers (cargo) come and go to and from the station (basal body) to ride on the trains, but the trains themselves simply go back and forth between stations, never leaving the tracks (flagellar outer doublets). It is also possible the exit of retrograde IFT particles from the base of the flagellum is tightly coupled with the entry of new IFT particles, such that an uninterrupted kymograph trace results. Distinguishing these two possibilities will require photobleaching analysis of particle turnover in live cells. These kymograph results have many caveats, the most serious being that one cannot tell precisely what a given DIC trace actually represents. We would most especially like to know what fraction of the total IFT proteins in the flagellum are present in the large visible traces, and what fraction are invisible to the method. Nevertheless, taking this data at face value, it is at least suggestive of a rather tight association of IFT complexes with outer doublet microtubules in vivo. Electron micrographs of cross sections through Chlamydomonas flagella invariably reveal the IFT particle aggregates as long chains of protein tightly apposed to the B tubule of the outer doublet. Given this intimate association of IFT particles with the outer doublets, data showing that particles move back and forth without leaving the doublet to which they are attached, and the fact that the number of IFT particle aggregates observed by immunofluorescence is approximately equal to the number of outer doublets in the flagellum, we propose a simple mechanism to control particle number. As illustrated in Fig. 2B, we suggest that each outer doublet interacts with a single IFT particle raft. This raft moves back and forth within the flagellar compartment, picking up new cargo at the base and depositing cargo at the tip, without ever leaving the flagellum. The IFT rafts thus behave analogously to elevators moving up and down in an elevator shaft. The entire flagellum thus behaves like an elevator core with nine elevator shafts. To keep the number of IFT particle rafts constant at nine per flagellum, it is only necessary

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Anterograde Tip

Basal body Ciliary membrane

Retrograde

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FIG. 2 Length‐independent regulation of intraflagellar transport—the elevator model. (A) Schematic of cilium, showing basal body embedded in cell cortex (purple) and ciliary membrane (green), which is topologically contiguous with plasma membrane but with a distinct lipid composition. IFT particles (red) are pulled by heterotrimeric kinesin‐II (gray) in the anterograde direction, and by cytoplasmic dynein (orange) in the retrograde direction. Cargo proteins such as tubulin are bound by the IFT particles and brought to the tip, where they are assembled onto the growing end of the axoneme. (B) Elevator model. Each outer doublet has a single IFT particle aggregate attached to it, which moves up and down from base to tip and back, like an elevator moving between floors. A defined copy number of nine aggregates per flagellum is thus attained if each doublet recruits exactly one aggregate. This could either be established during initial assembly or maintained by a timer that injects new particles onto unoccupied doublets.

for the flagellar pores (Deane et al., 2001) at the base of each doublet to monitor the presence or absence of an IFT particle raft on the doublet. A doublet lacking a raft would signal the pore to inject another IFT particle raft. The main feature of this model is that it solves the problem of how a flagellum can count to nine—it simply has to count to one, nine times. How does the flagellar pore recognize when it needs to inject an IFT particle? The simplest way would be for retrograde particles to interact with the pore in such a way as to inhibit further introduction of new IFT particles. This would explain why IFT particles accumulate in retrograde IFT mutants—although particles enter the flagellum, because they cannot return to the base, the

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flagellar pore ‘‘thinks’’ there is no particle raft on its corresponding outer doublet, so it lets in another bolus of IFT protein. This model easily accounts for the fact that retrograde IFT mutants accumulate IFT proteins in their flagella—the lack of returning retrograde particles would be interpreted by the flagellar pore as a lack of active IFT, and in response the pore would inject additional IFT particles, leading to an eventual accumulation. As previously mentioned, it is also possible IFT particles enter and exit the flagellum, but that entry and exit are coupled, and in this case the elevator model still works, because if entry of a new particle is coupled to exit of an old particle, the number of particles would never change. This alternate form of the model would, however, have diYculty accounting for the accumulation of IFT particles in a retrograde mutant. This model, which we emphasize is purely speculative at the moment, makes the prediction that length‐altering mutations could occur in components of the flagellar pore apparatus. One conceptual advantage of the balance‐point model is that the constant ongoing turnover could potentially allow rapid readjustment of length in response to cellular signaling cues. For instance, cells resorb their flagella prior to division. Studies in Chlamydomonas suggest that this resorption involves intraflagellar transport, either as a trigger for increased disassembly or severing (Parker and Quarmby, 2003) or as part of the disassembly machinery itself (Pan and Snell, 2005). We also note that in the balance‐point model, the basal body plays a key role, potentially controlling the entry of both IFT proteins and flagellar precursor proteins into the flagellum. Thus, modifications or regulation of activities localized to the basal body would be expected to result in changes in flagellar length. This could provide a simple explanation for the fact that many cell types can possess flagella of diVerent lengths depending on the maturation age of the corresponding basal bodies (Schoppmeier and Lechtreck, 2003).

IV. Conclusion: What Have We Learned from Flagellar Length Control? Although flagellar length control in the green alga Chlamydomonas is a fascinating biological puzzle, we anticipate that the lessons learned from studying this simple and tractable system will be readily extendible to other contexts. A. Length Control as Pharmacological Target for Ciliary Disease As noted in the first section of this review, ciliary diseases in humans are often characterized by short cilia, rather than a complete absence of cilia. The degree to which an abnormally short cilium is detrimental may depend on the function of

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the cilia in a particular tissue. For motile cilia, that need to move fluid via their own motility, reduced length is obviously a severe problem. The same is true of mechanosensory cilia, such as those of the kidney—a shorter cilium will have diVerent mechanical properties, and is likely to produce less bending at the base in response to a given rate of fluid flow. For chemosensory cilia, short or stumpy cilia may have less surface area into which receptors may embed. They may thus lack the sensitivity of a longer cilium. In all cases, shorter cilia are likely to have reduced, but not eliminated function. This partial function may be the reason the disease results in symptoms at all—a disease mutation resulting in a complete loss of cilia is most likely to be lethal in early development. Given that abnormal ciliary length may underlie many human ciliary diseases, what can we do about it? The fact that mutants with abnormally long cilia exist suggests that if pharmacological interventions can be devised to induce an increase in ciliary length, these could be used to treat ciliary diseases with short cilia. For instance, assuming the balance point is correct, a disease caused by a partial reduction in IFT, which would tend to cause a shortening of cilia, could be compensated by a chemical therapy that inhibits turnover. Similarly, the molecular signaling pathways that lead to increased length, such as the LF4 pathway, provide potential targets for drug development—a chemical inhibitor of LF4 ought to lead to an increase in ciliary length. To implement this general scheme for treating ciliary disease, there are two major requirements. First, it is important to determine the extent to which the length‐control machinery in human cells matches that of Chlamydomonas. This is simply a question of repeating, in human cells, the types of experiments described earlier in algae. It will be especially interesting to see whether reverse genetic knockdown of the human homologs of the LF genes will produce a similar increase in length of primary cilia. Second, eYcient and highly parallelizable assays will be needed to allow high throughput screening of compounds for a potential eVect on length. By combining green fluorescent protein (GFP) constructs specifically targeted to cilia, with automated high throughput imaging devices, it should be possible to rapidly screen through hundreds of thousands of compounds to identify candidates for further study.

B. Flagellar Length Control as Paradigm for General Organelles A major reason for studying flagellar length control is that the ease of analysis provided by this organelle makes it possible to do large numbers of simple experiments. The hope, however, is that the general models for length control derived from experiments in Chlamydomonas flagella will ultimately be applicable to size control of other types of organelles. First, we consider other organelles whose size can be described entirely by length. The most obvious is

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the microvillus. Microvilli contain parallel bundles of actin filaments. We have previously presented a simple model, analogous to the balance‐point model of flagellar length control, to account for length regulation in microvilli (Marshall, 2004). It is known that actin in microvilli undergoes continuous treadmilling, with retrograde movement of the filaments toward the cytoplasm balanced by continuous addition of new actin at the tip. It is also known that actin monomer reaches the tip via diVusion. Solution of the diVusion equation for a one‐ dimensional system at steady state with a constant rate of addition at the tip balancing constant treadmilling, results in a system that can achieve a unique, stable steady‐state value for its length (Marshall, 2004). This model is, in an abstract sense, very similar to the balance point model for flagellar length control. The only real diVerence is that the inherent length dependence of assembly derives not from the details of IFT, but rather from the dependence of monomer concentration on length at steady state. So far, this type of model has not yet been tested for microvilli, but there is no reason why it could not be tested. In fact, the very same methods that have been used to test the mechanism of flagellar length control in Chlamydomonas (Marshall and Rosenbaum, 2001; Marshall et al., 2005) can be directly applied to microvilli: specifically one would like to measure the assembly kinetics, resorption kinetics when assembly is blocked, and the dependence of length on number when multiple microvilli are forced to compete for a common pool of precursor. Genetics can also be used to probe the mechanism of length control in microvilli, by identifying partial loss‐ of‐function alleles in, for instance, the motors that drive treadmilling, and then comparing the observed phenotype with results of simulations. It remains to be seen how many other linear structures will have their length controlled by similar processes. For instance it now seems likely that the sarcomere size in striated muscle uses a very diVerent mechanism that may be based on a molecular ruler (Fowler et al., 2006). To ultimately conduct the same types of length control studies in other cellular systems, a major challenge is the fact that flagella are so much longer than most other linear structures. Fortunately, several clever new imaging and image processing methods have greatly facilitated precise and accurate length measurement for very small structures (Littlefield and Fowler, 2002), and it seems likely the development and application of these measuring tools, combined with reverse genetics and mathematical modeling, will soon lead to a clear understanding of length control in general, at which point it will be interesting to see what overall patterns emerge in the types of mechanisms that biology has evolved to control length. What about organelles that are not simple linear structures? So far, size control in such structures remains very poorly understood. We have previously proposed an abstract version of the balance point model which frees it from a single dimension (Marshall, 2002). To formulate such a model, which is really a schema for generating models rather than a specific model per se, we note that the balance‐point model for length control hinges on two

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features. First, the model requires the structure to be dynamic, such that size control works by setting the assembly and disassembly rates equal at a single value of size. Second, the model requires that assembly is inherently length dependent, due to the properties of IFT. To generalize from this specific model, we say that size control of an organelle can work by a balance‐point type of mechanism if two features are present: first, the organelle must be dynamic such that its size (surface area, volume, etc.) is constantly changing slightly as the result of ongoing assembly (e.g., via fusion of vesicles onto the organelle surface and budding of vesicles oV of the surface), and second, that either the assembly or disassembly rate, or both, is inherently size‐dependent. For instance, if a membrane‐bound organelle is exchanging vesicles with the ER (or any other large reservoir of material), then we can assume the rate of vesicles traveling to the organelle and fusing with its surface will depend only on the rate of vesicle formation at the ER and transit to the organelle, and not on the surface area of the organelle (because we presume the ER has no way of knowing how big the distant organelle actually is). If we further assume the rate of vesicle budding from the surface is proportional to the surface area, we immediately obtain a simple balance‐point model for size control. If we let the rate of vesicle fusion onto the surface be represented by the variable a, and the rate of budding be equal to bS, then the instantaneous rate of change of the surface area S is given by dS/dt ¼ a bS . If we solve for the steady state solution by setting dS/dt ¼ 0, we find that the system only can maintain a steady‐state surface area when S ¼ a/b. This steady‐state solution is stable, because if the surface area were to increase, now the budding rate would go up, leading to a reduction in area back down to the steady‐state solution. Similarly, if the area were to somehow be reduced, now assembly (fusion) would predominate and restore the organelle to its steady‐state size. This simple generalization of the balance‐point model seems reasonable but it has never been tested for any membrane‐bound organelle so far. Testing the model can proceed using the same methods developed for probing the mechanism of flagellar length control, such as measuring growth kinetics or the dependence of size on the number of organelles present in a given cell. We conclude that flagellar length control continues to serve as a valuable paradigm for studying the problem of organelle size control in general. The types of length control models resulting from the study of flagellar size provide insights into possible models that could regulate size in other systems. The experimental strategies that have been devised to study flagellar length can likewise be used to devise similar approaches for the study of other organelles. More generally, the fact that flagellar length control studies give us easy access to quantitative information which can be used for mathematical modeling, suggests that flagella will be a paradigm not just for size control, but for a more general systems‐biology approach to cellular structure.

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C. Length Control in Nanotechnology Current eVorts to build more complex and miniaturized machines using the methods of nanotechnology are faced with the same problems that the cell faces in building its substructures. How does one specify the size of the structure, or its position, or the number of copies to be made? Much current eVort in nanotechnology solves these problems using the type of fabrication processes used in building man‐made machines—a blueprint is developed that explicitly encodes all spatial information (size, position, etc.), and then this blueprint is used to direct the activity of a fabrication device, such as a lithographic process. Such methods reach a hard limit on size scale, imposed by the physics of the fabrication process. For instance, photolithography is limited in the size of the features it can produce, by the wavelength of the light used. An alternative method, currently under consideration, is self‐organization (Ewaschuk and Turney, 2006). In this paradigm, components of a nano‐machine would put themselves together. This type of fabrication gets around the normal physics‐imposed constraints, because there is no need to convert a macroscopic blueprint or image into a microscopic structure. Because self‐assembly of the type currently being considered for nanotechnology applications is precisely the fabrication principle used by cells, it makes sense to ask whether the methods employed by cells can be applied to human‐ designed nanomachines. Controlling the length of polymeric structures is a major issue in nanotechnology (Graveland‐Bikker et al., 2006). The same mechanisms employed for length control within cells (molecular rules, cumulative strain, quantal production, feedback, and balance‐point regulation) are all potentially applicable to length control in nanotechnology. Further, the axoneme itself is promising as a potential platform for the fabrication of very small machines. With its precise symmetry, and 96‐nm repeating arrangement of dynein arms, it provides a highly structured lattice on which other small components could be positioned. Pursuit of this specific approach to nano‐biotechnology will obviously require a very deep quantitative understanding of how the flagellum is put together. Length control is just one part of this understanding.

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Molecular Mechanism and Evolutional Significance of Epithelial–Mesenchymal Interactions in the Body‐ and Tail‐Dependent Metamorphic Transformation of Anuran Larval Skin Katsutoshi Yoshizato Department of Biological Science, Graduate School of Science, Hiroshima University, Higashihiroshima, 739‐8526, Japan

The epidermis of an anuran larva is composed of apical and skein cells that are both mitotically active and self‐renewed through larval life. In contrast, the epidermis of an adult frog, with typical stratified squamous epithelium composed of germinative basal, spinous, granular, and cornified cells, is histologically identical to the mammalian epidermis. Two important issues have not yet been addressed in the study of the development of anuran skin. One is the origin of adult basal cells in the larval epidermis and the other is the mechanism by which larval basal cells are transformed into adult basal cells in a region‐ (body‐ and tail‐) dependent manner. The cell lineage relationship between the larval and adult epidermal cells was determined by examining the expression profiles of several genes that are expressed specifically in larval and/ or adult epidermal cells and differentiation profiles of larval basal cells cultured in the presence of thyroid hormone (TH). Histological analyses using several markers led to the identification of the skin transformation center (STC) where the conversion of larval skin to the adult counterpart is taking place. The STC emerges at a specific place in the body skin and at a specific stage of larval development. The STC progressively ‘‘moves’’ into and ‘‘invades’’ the adjacent larval region of the trunk skin as a larva develops, converting the larval skin into the preadult skin, but never into the tail region. The larva to preadult skin conversion requires an epidermal–mesenchymal interaction. The genesis of preadult basal cells is suppressed in the tail epidermis due to the influence of underlying mesenchyme in the tail region. PDGF signaling is one of the molecular cues of epidermal–mesenchymal interactions. In addition, a unique feature of

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0074-7696/07 $35.00 DOI: 10.1016/S0074-7696(06)60005-3

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anuran skin metamorphosis is presented referring to the skin of other vertebrates. Histological comparisons of the skin among vertebrate species strongly suggested a similarity between the anuran larval skin and the teleost fish adult skin and between the anuran adult skin and the adult skin of other tetrapod species. Based on these similarities, the evolutional significance of anuran skin metamorphosis is proposed. Finally, studies are reviewed that reveal the molecular mechanism of anuran metamorphosis in relation to TH‐TR‐TRE signaling. The results of these studies suggest new aspects of the biological significance of TH, and also enable us to envision concerted regulations of the expression of a gene in the frame of the gene network responsible for metamorphic remodeling of larval tissues. The present review will contribute to an understanding of the molecular mechanism of region‐dependent skin development of anurans from not only a metamorphic but also from an evolutional point of view, and will provide a new way to understand the biological significance of TH in anurans. KEY WORDS: Thyroid hormone, Rana catesbeiana, Epidermal basal cells, Tissue remodeling, Vertebrate skin, Thyroid hormone response element. ß 2007 Elsevier Inc.

I. Introduction After fertilization, anurans undergo embryogenesis, larval development, and metamorphosis to adults. To meet the change in habitation from the aquatic to terrestrial environment, the larva undergoes extensive postembryonic remodeling of most of its tissues in which the cells required only for larval life undergo apoptosis. In contrast, the cells required for adult life diVerentiate into adult cells. A larval tissue composed of larval cells develops into an intermediate and transient tissue in which adult progenitor cells (preadult cells) newly emerge (Fig. 1). Thus, the tissue becomes chimeric in that preadult cells and larval cells coexist. Preadult cells diVerentiate into adult cells, whereas larval cells undergo apoptosis and disappear from the tissue during metamorphosis. Therefore, there are two populations of larval cells: one (larva‐proper cells) that terminates its lineage at metamorphosis and the other whose lineage is maintained as adult cells. A. Region‐Dependent Progression of Skin Remodeling in Anuran Metamorphosis The larval epidermis is one of the tissues that has been extensively studied in terms of the mechanism underlying such a metamorphic transformation of larval cells. The epidermis has an additional uniqueness that attracts us:

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Metamorphic stage FIG. 1 Two types of larval cells with diVerent diVerentiation potentials. Cellular events are shown that take place during larval to adult development. A larval tissue at an early developmental stage (premetamorphic stage) contains cells with diVerent diVerentiation potentials and develops into an intermediate tissue, in which some cells are committed to diVerentiate into preadult cells (adult progenitor cells) in a middle stage of development (pro‐ and premetamorphic stage), whereas other cells remain as larval cells. The preadult cells diVerentiate into adult cells that form adult tissue in a late stage of development (climax stage of metamorphosis). Larval cells undergo apoptosis, thus their lineage is being terminated.

the metamorphic program of the epidermis is quite diVerent between the cephalic part (head and trunk region and then the body) and the caudal part (tail region). Among epidermal cells, basal cells that attach themselves to the basement membrane play prime roles in constructing the epidermis. The body and tail basal epidermal cells undergo a ‘‘transformation program’’ and an ‘‘apoptosis program,’’ respectively. Common larval cells construct larval epidermis in both the body and the tail regions of a tadpole in an early stage of development (Fig. 2). Then, the epidermis in the body becomes chimeric containing both larval and preadult cells, which then follows the two diVerent metamorphic programs (transformation and apoptosis) under the same hormonal (thyroid hormone, TH) cue. In contrast, the tail epidermal cells do not diVerentiate into preadult cells, but remain larval in nature through the end of metamorphosis, and undergo apoptosis. This apoptotic event in the tail is really massive and of a large scale, because the tail region just before the onset of metamorphosis occupies 33% and 25% of the total length and the volume of a tadpole of Xenopus laevis, respectively. The major aim of this review is to present a current view of how the originally homogeneous epidermal basal cell population becomes heterogeneous in its diVerentiation potential in a region‐ and TH‐dependent manner. The studies accumulated in our laboratory on skin metamorphosis have led us to hypothesize the presence of a metamorphic skim transformation center (STC) where interactions between the epidermis and the subepidermal connective tissue induce the larval skin to transform into its adult counterpart. STC is not formed in the tail region.

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Body

Larval

Tail

Body

Tail

Intermediate

Body

Adult

Metamorphic stage FIG. 2 Two types of epidermal basal cells with regional diVerences. There are no diVerences in phenotypes of basal cells in the larval epidermis between the body and tail regions. Some basal cells in the body transform into preadult basal cells (adult progenitor cells) in the intermediate stage, but those in the tail do not show such a transformation. The preadult cells diVerentiate into adult basal cells and construct the adult epidermis. Larval cells in both regions undergo apoptosis. The symbols in the illustration are as in Fig. 1. The horizontal bar underneath the cells represents the basement membrane. The dotted vertical line represents the boundary between the body and the tail regions. The symbols for the cells are used as in Fig. 1.

B. Evolutional Significance of Anuran Skin Metamorphosis When skin histology was compared among the teleost, the anura, and the mammal, we noticed the similarity between the anuran larva and the fish adult and between the anuran adult and the amniote adult. These similarities appear to be correlated with the environmental diVerences in the habitation of these animal species. Therefore, we speculate that anuran skin metamorphosis is a process that might have taken place when ancestral anurans evolved from fish approximately 350 million years ago. It could be said that the metamorphic process of the anuran skin recapitulates the evolutionary process from the aquatic life of teleost fish to the terrestrial life of tetrapods.

C. Regulation of Metamorphosis by Thyroid Hormone TH triggers metamorphosis of an anuran larva and induces its transformation to the adult. Larval cells receive TH with the nuclear TH receptor (TR). TR acts as a transcription factor by binding to the TH response element (TRE) of metamorphosis‐associated and TH‐direct responsive genes. This flow of the TH‐TR‐TRE signal in larval cells plays a key role in anuran metamorphosis. It has generally been considered that the biological significance of TH in anurans resides solely in its metamorphosis‐inducing activity (metamorphosis hormone), because TH in serum is detectable only during

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217

climactic stages of metamorphosis. Studies have been accumulated in which the molecular mechanism of anuran metamorphosis was examined in relation to TH‐TR‐TRE signaling. We obtained evidence that suggests that TH plays roles not only in metamorphosis, but also in embryogenesis and in physiological processes of adult tissues. Studies on amphibian metamorphosis at the molecular level have revealed the regulation of the expression of individual metamorphosis‐associated genes. Accumulation of these studies will permit us to envision concerted regulation of gene expression in the frame of gene networks that govern the metamorphic remodeling of larval tissues.

II. Anuran Skin Remodeling and Metamorphosis A. Development of Anuran Skin from the Late Embryonic Stage to the Adult The skin of Rana catesbeiana and Xenopus laevis larva is homologous in histological structures, but develops diVerently in chronology as shown in Fig. 3A and B, respectively. The larva to preadult skin conversion takes place early (at a premetamorphic stage) in larval life around stage IV (TK‐IV), defined by Taylor and Kollros (1946) in R. catesbeiana (Kawai et al., 1994; Suzuki et al., 2001, 2002; Utoh et al., 2000), but much later (at a prometamorphic stage) around stage 58–59 (NF‐58–59) defined by Nieuwkoop and Faber (1967) in X. laevis (Utoh et al., 2003; Watanabe et al., 2001, 2002). Various epidermal cell species are involved in the development and metamorphosis: basal skein, suprabasal skein, larval basal, preadult basal, adult basal cells, and diVerentiated descendants of adult basal cells (Izutsu et al., 1993; Suzuki et al., 2001, 2002; Utoh et al., 2000, 2003; Watanabe et al., 2001, 2002; Yoshizato, 1996). Apical cells are located at the outermost layer. Skein cells are defined as the larval epidermal cells that contain in the cytoplasm conspicuous spirally wound tonofilaments taking the appearance of huge bundles of intermediate filaments called ‘‘Figures of Eberth’’ (Eberth, 1866; Fox, 1992; Fox and Whitear, 1986). These cells are so called because this unique keratin bundle possesses ‘‘skein,’’ a loosely coiled length of thread wound on a reel. Skein cells are a major cell type of anuran larval epidermis (Yoshizato, 1989). Rana larval keratin (RLK) is a component of keratin bundles and thus a useful biochemical indicator of skein cells (Suzuki et al., 2001). Xenopus larval keratin (XLK) is a Xenopus homologue of RLK (Watanabe et al., 2001). There are two types of skein cells: basal and suprabasal skein cells. Electron microscopic observations showed that basal skein cells apparently resemble larval basal cells (Izutsu et al., 1993). However,

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these two types of cells are morphologically quite diVerent from each other in that the basal skein cells, but not the larval basal cells, do contain keratin bundles. Apical and suprabasal skein cells undergo TH‐induced apoptosis, whereas larval basal cells proliferate in response to the stimulus of the same hormone (Nishikawa et al., 1989; Yoshizato, 1996). Larval basal cells are present in the trunk (hereafter, body), but rarely in the tail (Izutsu et al., 1993). Orthogonally arranged multilayered collagen fibers (collagen layer or lamella) beneath the basement membrane feature the amphibian subepidermal connective tissue (Utoh et al., 2000; Weiss and Ferris, 1954; Yoshizato, 1989). These collagen lamellae are formed by type I collagen originally synthesized by basal skein cells and later also by subepidermal fibroblasts (Utoh et al., 2000).

ap

A

X

oc

Gosner 22

ss

ic mes

lb

TK-I

bs fi

s-ct p-ct

fi ap

II

cl bs cl

fi

p-ct

p-ct

XXII

III

gr

ap ss

sp

bs

ab cl

IV

s-ct

gl

p-ct

fi co

Froglet

ap

ss

gr

lb

sp gl

s-ct cl fi

p-ct

s-ct

ab

219

EPITHELIAL–MESENCHYMAL INTERACTION IN ANURAN LARVAL SKIN

B

NF 35 58

oc

ap

ic

ss

mes gl cl

lb

s-ct p-ct

40

ap

62

bs

gr sp cl ap

gl

ss

Froglet

co gr

bs p-ct

fi

ab

p-ct

51 cl

s-ct

sp ab

ap

ss

bs

s-ct

54 cl p-ct

FIG. 3 Comparison of the development of skin between Rana catesbeiana and Xenopus laevis. Histology of skin of Rana catesbeiana (A) and Xenopus laevis (B) at the indicated developmental stages, sectioned, and stained with hematoxylin and eosin. oc, outer cell; ic, inner cell; mes, mesenchyme; bs, basal skein cell; p‐ct, p‐connective tissue; fi, fibroblast; ap, apical cell; cl, collagen lamella; ss, suprabasal skein cell; lb, larval basal cell; s‐ct, s‐connective tissue; gr, granular cell; sp, spinous cell; co, cornified cell; ab, adult basal cell; gl, gland. Bars, 50 mm.

The epidermis of Rana embryos at a late embryonic stage, stage 22 after Gosner (1960), is composed of two‐cell layers, outer and inner layers (Fig. 3A). The epidermis of larvae just after hatch (TK‐I) is one‐cell layered (Utoh et al., 2000) and then becomes two‐cell layered at late TK‐I, with apical and basal skein cells in the upper and inner layer, respectively. It becomes three‐cell layered at TK‐III, the upper, middle, and lower layer consisting of apical, suprabasal skein, and basal skein cells, respectively (Suzuki et al., 2001; Utoh et al., 2000). The larval basal cells first emerge at around TK‐IV (Utoh et al., 2000), a critical event because the larval basal cells were considered to be a progenitor of adult basal cells (Robinson and Heintzelman, 1987; Yoshizato, 1996).

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Initially (TK‐I to ‐III), the subepidermal basement membrane directly contacts the acellular collagen layer that is associated with ‘‘primary connective tissues’’ (p‐connective tissues, Fig. 3A). Concomitantly with the emergence of larval basal cells ‘‘secondary connective tissues’’ (s‐connective tissues) are formed between the basement membrane and the collagen lamella at a late early premetamorphic stage (around TK‐IV; Utoh et al., 2000). Collagen lamellae are populated with fibroblasts. This event takes place in the STC as detailed in Section V. Through these changes, the larval skin transforms into the ‘‘preadult skin,’’ the skin containing larval basal cells and s‐connective tissue. The preadult skin develops, increasing the number of intermediate cell layers and the area of s‐connective tissues until the onset of the climax stage (TK‐XX). During the climax stages, the preadult skin is transformed into the adult skin, deleting suprabasal skein and apical cells, and diVerentiating larval basal cells to their adult counterparts. Xenopus larvae have a two‐cell layered epidermis from the late embryonic stage through the hatching stage (NF‐stage 35): the outer and the inner layer (Fig. 3B). The epidermis then develops into a larval type composed of apical and basal skein cells around NF‐40. Suprabasal skein cells have appeared at NF‐51. Collagen lamellae become prominent around NF‐54. Drastic changes in the skin take place at NF‐58, a late prometamorphic stage. The larval skin converts to the preadult skin. Preadult basal cells emerge and the s‐connective tissues are formed between the basement membrane and the acellular collagen layer. Thus, the skin at NF‐58 of Xenopus larvae corresponds to that at TK‐IV of R. catesbeiana. The preadult skin is eventually transformed into the adult skin at the completion of metamorphosis.

B. Molecular Probes for Anuran Epidermal Cells Appropriate molecular markers have been sought for or newly identified to investigate the lineage relationship among these diVerent types of anuran epidermal basal cells. For this, the following four genes/proteins are particularly useful: integrin b1, collagen a1(I) (COLa1), RLK, and Rana adult keratin (RAK). Integrin b1 is expressed in mammalian epidermal stem cells located in the basal layer and controls the diVerentiation of keratinocytes (Jones and Watt, 1993; Jones et al., 1995; Watt, 2001). Rana epidermal basal cells commonly express this gene from larval to adult life (Suzuki et al., 2002). Collagen type I is usually expressed in mesoderm‐derived tissues such as bones and dermis of adult mammals. However, interestingly, it was found that its gene (cola1) is expressed in the inner layer of epidermis during Xenopus embryonic development (Goto et al., 2000). We cloned bullfrog COLa1cDNA (Asahina et al., 1997) and showed that this unique expression continued to early larval development (Suzuki et al., 2002; Utoh et al., 2000).

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EPITHELIAL–MESENCHYMAL INTERACTION IN ANURAN LARVAL SKIN

The inner epidermal cells at Gosner stage 23 expressed the cola1. The epidermis at the early TK‐I is one‐cell layered and these cells expressed it. These single‐layered epidermal cells produce two types of cells: apical cells and basal skein cells. Only the latter cells express cola1. The basal skein cells yield suprabasal skein cells at TK‐III that do not express the gene. Larval basal cells do not express cola1. Thus, cola1 is a specific and unique gene marker of embryonic to early‐larval basal epidermal cells. RLK and XLK are of type II keratin and each is a member of the proteins consisting of Figures of Eberth of Rana (Suzuki et al., 2001) and Xenopus (Watanabe et al., 2001), respectively. XLK was originally found as a protein on two‐dimensional electrophoretic gels for the larval skin proteins (Kobayashi et al., 1996); it was sequenced and its cDNA was cloned (Watanabe et al., 2001). RLK cDNA (rlk) was cloned using specific antisera against XLK (Suzuki et al., 2001). A subtractive cloning between the body and the tail skin of bullfrog tadpole yielded a cDNA (rak) of RAK (Suzuki et al., 2001). Adult‐type keratin cDNAs of X. laevis were screened from an adult skin cDNA library using probes that were designed from the highly conserved N‐terminal of the rod domain of type I keratin, which resulted in yielding three types of xak, xak‐a, ‐b, and ‐c (Watanabe et al., 2001, 2002). Among them, xak‐c is expressed in basal cells (Watanabe et al., 2002). The other two keratins are present in granular and spinous cells (Watanabe et al., 2001). RAK and XAK are of type I keratin. Granular cells of Rana species also express specific cell surface antigens that react with antihuman blood group A antigen (hbA) antibodies (Izutsu et al., 1993). Table I summarizes the distributions of these markers among epidermal cells of anurans together with mammals for the sake of comparison. TABLE I Molecular Probes for Anuran and Mammalian Epidermal Cells Rana catesbeiana

Xenopus laevis

Homo sapiens

RK8

XLK19a

CK8, CK18b

Skein cell

RLK

XLK

–

Basal skein cell

RLK, COLa1, SPARC, integrin b

XLK, SPARC

–

Larval basal cell

RLK, RAK, integrin b

XLK, XAK‐C

–

Adult basal cell

RAK, integrin b, SPARC

XAK‐C, SPARC

CK5, CK14, integrin b

Spinous/granular cell

hbA

XAK‐A, XAK‐B

CK1, CK10

Apical cell (periderm)

a

Furlow et al. (1997). Moll et al. (1982).

b

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KATSUTOSHI YOSHIZATO

Figure 4 shows the expression of cola1, rlk, and rak in respective cells during the metamorphosis of bullfrog tadpole, at early TK‐II, ‐III, ‐X, and adult. Fluorescent views of Bouin‐fixed sections are also presented to identify Figures of Eberth (Kawai et al., 1994). Basal skein cells at early TK‐II express COLa1 (Fig. 4A) and RLK (Fig. 4B), but not RAK mRNAs (Fig. 4C). Basal skein cells have not developed keratin bundles (Fig. 4D). The skin at TK‐III shown in Fig. 4E contains suprabasal skein cells and the fibroblast‐populated collagen lamella. Fibroblasts are concentrated near the lamella. These fibroblasts intensely express cola1. The basal cells well develop keratin bundles (Fig. 4H) and intensely express cola1 (Fig. 4E) and rlk (Fig. 4F). Importantly, these cells do express RAK mRNA, an adult basal marker gene (Fig. 4G), indicating that basal skein cells proceed to the next step of basal cell diVerentiation. We call the basal skein cells at this step ‘‘rakþ basal skein cells’’ to emphasize that the basal skein cells begin to express an adult gene. Thus, the rakþ basal skein cells are defined as the cells that express genes of cola1, rlk, and rak, and contain keratin bundles. The suprabasal skein cells express rlk (Fig. 4F). The dermis at TK‐X contains s‐connective tissues (Fig. 4I–L). Basal cells cease to express cola1 (Fig. 4I) and rlk (Fig. 4J), and do not contain keratin bundles (Fig. 4L), indicating that the basal cells drastically change their characteristics. They discard several larval traits, but continue to express rlk and rak (Fig. 4K). We call these basal cells ‘‘larval basal cells’’ or ‘‘preadult basal cells,’’ and propose using the term ‘‘preadult skin’’ as the skin that contains larval basal cells in the epidermis and the s‐connective tissue in the dermis. Suprabasal skein cells at TK‐X abundantly propagate and form multilayers, and their keratin bundles are conspicuous (Fig. 4L). The adult basal cells do not express cola1 (Fig. 4M) and rlk (Fig. 4N), but do express rak (Fig. 4O). The epidermis does not contain suprabasal skein cells (Fig. 4P). The previously mentioned expression profiles of the molecular markers for various types of basal cells strongly suggest a pathway of their development and diVerentiation during metamorphosis as shown in Fig. 5. Presently, at least four types of basal cells have been distinguished in the epidermis during larval and metamorphic development. These cells sequentially emerge on the basement membrane during development of a tadpole as follows: basal skein cells, rakþ basal skein cells, larval (or preadult) basal cells, and adult basal cells. They are considered to be on the same lineage (Suzuki et al., 2002). Skein cells are the cells that contain keratin bundles (kbþ) and express cola1 and rlk, but not rak (kbþ, cola1þ, rlkþ, rak ). Rakþ basal skein cells are of kbþ, integrin b1þ, cola1þ, rlkþ, and rakþ. Larval basal cells are of kb , integrin b1þ, cola , rlkþ, and rakþ. Adult basal cells are of integrin b1þ, cola1 , rlk , and rakþ.

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EPITHELIAL–MESENCHYMAL INTERACTION IN ANURAN LARVAL SKIN

TK-II

III

X

Adult

A

E

I

M

B

F

J

N

C

G

K

O

D

H

L

P

colα1

rlk

rak

KB

FIG. 4 Distribution of mRNAs of COLa1, RLK, and RAK in the epidermis. In situ hybridization was performed with cRNA probes of COLa1 (cola1) (A, E, I, M), RLK (rlk) (B, F, J, N), and RAK (rak) (C, G, K, O) for the Rana epidermis at TK‐II (A, B, C), III (E, F, G), X (I, J, K), and adult (M, N, O). Bouin‐fixed skin sections (KB) are shown for TK‐II (D), III (H), X (L), and adults (P). Arrowheads in the figures point to some of the basal cells. (A) The COLa1 gene is expressed in basal skein cells (bs), but not in apical cells (ap). Fibroblasts in p‐connective tissues (p‐ct) also weakly express the gene (arrows). No fibroblasts are in the collagen lamella (cl). (B) The RLK gene is expressed in basal skein cells, but not in apical cells. (C) RAK mRNA is not detected in any cells. Brown and red colors represent pigment cells. (D) Strong fluorescence is seen in the collagen lamella (cl). The two‐layer structure of the epidermis is clearly recognized and basal skein cells do not develop keratin bundles. (E) Basal cells intensively express cola1 (arrowheads). Collagen lamellae are invaded by fibroblasts (#). These fibroblasts and the fibroblasts (##) approaching the lower side of the collagen lamella strongly express cola1. (F) RLK mRNA is detected in both suprabasal skein (ss) and rakþ basal skein cells but not in apical cells. (G) RAK mRNA is observed only in rakþ basal skein cells (arrowheads). (H) The three‐layer structure is clearly seen in the epidermis. Keratin bundles (kb) are well developed in two types of skein cells, rakþ basal skein cells and suprabasal skein cells. (I) Laval basal cells (lb) do not express cola1. The s‐connective tissue (s‐ct) is formed between the basement membrane and the collagen lamella. The collagen lamella and p‐connective tissue (p‐ct) are not seen here and in (J) through (P). (J) Suprabasal skein cells, but not apical and larval basal cells, express rlk. (K). Larval basal cells, but not apical and suprabasal skein cells, express rak. (L) Suprabasal skein cells fully develop fluorescent keratin bundles. (M) No signals of COLa1 mRNA are seen in the adult epidermis. c, cornified cells; ab, adult basal cells. (N) RLK mRNA is not detected in the adult epidermis. (O) RAK mRNA is exclusively and intensively expressed in adult basal cells (ab). (P) Keratin bundles are not observed in adult epidermal cells. Bar, 50 mm.

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KATSUTOSHI YOSHIZATO

Basal skein cells

rak + basal skein cells

Larval basal cells

Adult basal cells

BM Integrin b1

Gene expression

Collagen a1 (I) RLK RAK

FIG. 5 Sequential changes of types of anuran basal epidermal cells during metamorphosis. Basal skein cells are defined as the cells that express cola1 and rlk, and have keratin bundles. When basal skein cells start to express rak, we call them rakþ basal skein cells. rakþ basal skein cells diVerentiate to larval basal cells by losing keratin bundles and terminating cola1 expression. Finally, larval basal cells diVerentiate into adult basal cells by terminating the expression of RLK. The rectangles represent the period of time of their expression. The expression of the gene of integrin b1, collagen a1(I), RLK, and RAK is shown in green, white, yellow, and deep pink, respectively. The cell‐attached long thin bar represents the basement membrane (BM). The double yellow‐colored crescents that cross each other represent keratin bundles. The small gray‐colored ovals at the basal side of each of the cells represent integrin b1. The yellow and pink colors in the cytoplasm represent RLK and RAK, respectively. The gray rectangles and ovals enclosed by dashed lines indicate that the expression of integrin has not been determined yet.

C. Evidence That Basal Cells Include Epidermal Stem Cells and Larval Basal Cells Possess the Potential to Differentiate into Adult Counterparts Two possibilities have been put forward about the origin of adult basal cells (Yoshizato, 1986, 1989, 1992, 1996). (1) Larval and adult basal cells are on the same cell lineage: some of the larval cells diVerentiate into adult cells during metamorphosis. (2) Progenitor cells of adult basal cells diVerent from larval basal cells in cell lineage are present in the larval skin. Larval basal cells undergo apoptosis and progenitor cells of adult basal cells are activated and start to proliferate and diVerentiate into adult basal cells during metamorphosis. We tested which of the two possibilities works in both R. catesbeiana and X. laevis. The results obtained strongly supported the first possibility.

1. Studies on Rana Tadpole A one‐layered epidermis sheet composed only of preadult basal cells was prepared and cultured to examine the replication capacity and the diVerentiation potential of the basal cells (Suzuki et al., 2002). This experiment

EPITHELIAL–MESENCHYMAL INTERACTION IN ANURAN LARVAL SKIN

225

demonstrates two important aspects of basal cells: larval basal cells act as epidermal stem cells that are able to replicate and produce diVerentiated oVspring located in suprabasal layers, and larval basal cells are the origin of adult basal cells that are able to construct the adult epidermis. Pieces of Rana back skin were isolated from tadpoles at around TK‐X. Apical and suprabasal skein cells were completely removed from the skin by immersion in 70% ethanol and were shaken with Ca2þ‐ and Mg2þ‐free phosphate‐buVered saline containing 2.5 mM EDTA (Niki and Yoshizato, 1986). The skin sheets obtained are composed of the epidermis, which contains only larval basal cells, the basement membrane, and the dermis, consisting of the s‐connective tissue, collagen lamella, and the p‐connective tissues. These sheets were cultured for 9 days in the presence of aldosterone (AL), T3, or prolactin (PRL) (Fig. 6). Figure 6A–C clearly shows that the epidermis before culture (0 day) is a single layer composed of RLKþ and RAKþ larval basal cells (Fig. 6A, C). hbA‐positive cells are not present (Fig. 6B). The single‐layered epidermis develops into a multilayered epidermis (Fig. 6F). The basal layer is RLK and RAKþ (Fig. 6D), and the upper layers become intensely hbAþ (Fig. 6E). Importantly, AL alone is capable of inducing the diVerentiation of larval basal cells into adult basal cells. However, the epidermis is not a ‘‘true adult’’ epidermis, because its upper layers are RLKþ (Fig. 6D), indicating that AL induces the formation of unusual progenies in terms of protein profiles, simultaneously expressing both larval and adult proteins. Addition of T3 to the cultures does not aVect the expression of RAK in the basal layer (Fig. 6G), nor the expression of hbAþ (Fig. 6H), but, importantly, T3 terminates the expression of RLK in the upper layers (Fig. 6G). Thus, the epidermis becomes the ‘‘true’’ adult epidermis. An H&E‐stained section shows that the skin is of an adult type (Fig. 6I). It should be noted that basal, but not suprabasal cells require T3 to terminate the expression of RLK. On the other hand, the presence of PRL permits the basal cells to continue to be RLKþ and RAKþ as in day 0 cultures (Fig. 6J), supporting the notion that PRL is a stimulator of larval phenotype expression (Asahina et al., 1997). PRL induces the single layer of larval basal cells to form RLKþ and hbA suprabasal layers (Fig. 6J, K), its histology being of a larva type (Fig. 6L). This indicates that RLKþ suprabasal cells are progenies of larval basal cells. PRL inhibits the action of aldosterone to induce the diVerentiation of larval basal cells into adult basal cells and might stimulate the replication of larval basal cells, which results in the production of RLKþ cells. The hormone‐induced in vitro epidermal remodeling is schematically summarized in Fig. 6M. AL alone is capable of inducing the diVerentiation of larval basal cells into adult basal cells by terminating the expression of RLK. However, interestingly, RLK adult basal cells yield RLKþ suprabasal cells

226

KATSUTOSHI YOSHIZATO

RLK/RAK

hbA

H&E

A

B

C

D

E

F

G

H

I

J

K

L

0 day

AL

AL + T3

9 days

AL + PRL

Reconstruction of a "pseudoadult" epidermis

M AL Adult basal cell AL + T3

Larval basal cell

Reconstruction of a adult epidermis Adult basal cell Reconstruction of a preadult epidermis

AL + PRL Larval basal cell

FIG. 6 DiVerentiation capacity of larval basal cells of Rana catesbeiana into adult counterparts. Back skin sheets at TK‐X whose epidermis was composed of basal cells alone were cultured for 9 days in the presence of aldosterone (AL) (D, E, F), AL and T3 (G, H, I), or AL and PRL (J, K, L): the concentration of AL, T3, and PRL was 1 mM, 10 nM, and 2 mg/ml, respectively. The cultured skins were subjected to double immunohistochemical staining for RLK (red) and

EPITHELIAL–MESENCHYMAL INTERACTION IN ANURAN LARVAL SKIN

227

in this hormonal condition. T3 normalizes this unusual diVerentiation. Each of the apical and skein cells showed high [3H]thymidine‐labeling indices (Robinson and Heintzelman, 1987), suggesting that there are no hierarchical ‘‘stem cell to its progeny relationship’’ among basal cells and suprabasal cells in the tadpole skin. The results of the in vitro organ culture experiments demonstrate the presence of a hierarchical relationship in amphibian epidermis in the larva and the adult. The monolayered epidermis composed of larval basal cells reconstructed multilayered epidermis composed of hbAþ granular and cornified cells in the presence of AL and T3, which indirectly indicates that adult basal cells contain a stem cell population as in adult mammals (Watt, 2001). The monolayered epidermis is also able to construct multilayered epidermis composed of RLKþ suprabasal cells in the presence of AL alone, or AL and PRL. These RLKþ cells are most likely suprabasal skein cells. If so, this fact indicates that larval basal cells are able to construct the larval epidermis lacking apical cells. Thus, it is most likely that there is a mammalian type hierarchical relationship between basal skein cells and suprabasal skein cells, and between rakþ basal skein cells and suprabasal skein cells at each corresponding developmental stage of the larval epidermis. Apical cells are thought to be independent of ‘‘this stem cell to progeny lineage,’’ because there are no morphological and biochemical similarities among apical cells and the remaining epidermal cells (Furlow et al., 1997; Robinson and Heintzelman, 1987; Suzuki et al., 2001). Apical cells are highly mitogenic and are likely self‐replicative (Robinson and Heintzelman, 1987).

RAK (green) (RLK/RAK) (A, D, G, J). Or, they were subjected to single immunostaining for hbA (red) (B, E, H, K). Sections of skin were also stained with H&E (C, F, I, L). Sections of (A) through (C) are before culture (0 day). Photographs (in A, D, G, and J) are overlays of RLK and RAK stains. Double positive cells are seen in yellow. All the cells attached to the basement membrane indicated by the dashed lines were double positive before culture (0 day) (A) and in the cultures with AL and PRL (9 days) (J). Arrows in the H&E sections point to basement membrane. The abbreviations used are as in Fig. 4. Bar in (K), 50 mm. (M) A scheme for the hormonal regulation of the diVerentiation of larval basal cells. When larval basal cells are exposed to AL, they terminate RLK (yellow) expression and diVerentiate into RAKþ(pink) adult basal cells that produce hbAþ granular cells. Thus, larval basal cells are potentially progenitors of adult basal cells (adult epidermal stem cells), but cannot construct the ‘‘true’’ adult epidermis, because the progenies produced are RLKþ as well as hbAþ (‘‘pseudoadult’’ epidermis). The exposure of larval basal cells to both AL and T3 terminates the expression of RLK in the progenies, making the reconstructed skin the ‘‘true’’ adult skin. On the other hand, larval basal cells do not diVerentiate into adult basal cells when exposed to AL and PRL, but stay as larval basal cells and produce RLKþ progenies (most probably suprabasal skein cells). Pairs of green ovals at the base of cells represent integrin b1. Thus, it is concluded that larval basal cells also act as larval epidermal stem cells and construct the preadult epidermis. Taken together, larval basal cells potentially go into the two diVerent diVerentiation paths, the larval and adult path, depending on the hormonal environment. PRL enables larval basal cells to remain in the larval path. T3 forces the same cells to go into the adult path.

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2. Studies on Xenopus Tadpole Basically similar remodeling of larval to adult skin was reproduced in vitro in the presence of TH for Xenopus larval skin (Utoh et al., 2003). The back skin at NF‐54/55 whose epidermis is at a preadult stage was cultured for 9 days in the presence of AL, corticosterone, and hydrocortisone (Fig. 7). The epidermis before culture consists of apical cells at the surface, relatively large skein cells at the base, and small larval basal cells scattering among large skein cells at the base (Fig. 7A). The mesenchyme contains the collagen layer and p‐connective tissues. The larval basal cells are XLKþ (Fig. 7B) and XAK‐B and ‐C . Skin tissues remain larval when cultured without T3 for 9 days (Fig. 7C) except that aggregates of larval basal cells are formed. These aggregates are most likely to develop into secretory glands in the adult skin and are called the presumptive secretory gland (PSG). The skein and larval basal cells are XLKþ (Fig. 7D). There are no XAK‐Bþ cells (Fig. 7E). Notably a few XAK‐Cþ basal cells (preadult basal cells) are present around PSGs (Fig. 7E, arrows), suggesting that larval basal cells around PSGs are able to diVerentiate into preadult basal cells without TH. Skein and apical, but not basal, cells are mitotically active (Fig. 7F). The larval skin histologically diVerentiates into a near‐complete adult skin when cultured in the presence of T3 except that s‐connective tissue is not formed (Fig. 7G). Subepidermal fibroblasts appear to be activated, because, first, collagen lamellae markedly thicken and, second, multiple fibroblasts penetrate into the collagen lamella. There are no XLKþ cells (Fig. 7H). XAK‐Cþ adult basal cells increase greatly to a degree at which these cells occupy the whole region of the basal layer (Fig. 7I). Comparison of Fig. 7E and I suggests that the proliferation of preadult basal cells and their diVerentiation into adult basal cells are TH‐dependent processes. The upper layers contain XAK‐Bþ cells (Fig. 7I). Adult basal cells are in S‐phase of the cell cycle (Fig. 7J). This study clearly shows that originally XLKþ larval basal cells terminate the expression of xlk and instead start to express the xak‐c gene without T3, which represents the process of T3 ‐independent diVerentiation of larval basal cells into preadult basal cells as in R. catesbeiana. These active changes in the epidermal compartment are well associated with those in the mesenchymal compartment, both requiring TH. The in vitro organ culture experiments of larval skin of both Rana and Xenopus clearly demonstrate that larval basal cells actually have the potential to diVerentiate into adult basal cells. At present, the other important issue that remains to be clarified is whether basal skein cells actually have the potential to diVerentiate into larval basal cells. However, we previously presented indirect evidence that they have this potential (Yoshizato et al., 1993). Larval basal and basal skein cells were isolated from the back and the tail of Rana tadpoles at TK‐X, respectively, and cultured for 4 days in the

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FIG. 7 Larval to adult skin transformation in Xenopus laevis. (A–J) Pieces of back skin at stage 54/55 (A, B) were cultured for 9 days in the absence ( T3) (C–F) or presence of 100 nM T3 (þT3) (G–J). (A, C, G) H&E stains. (B, D, H) Immunostaining for XLK. (E, I) Double immunohistochemical staining for XAK‐C (red) and XAK‐B (green). (F, J) Skins were labeled with 20 mM BrdU for the last 24 h and were immunostained for BrdU. Dashed lines in the photographs represent the location of the basement membrane. Arrows with closed arrowheads in (E) show XAK‐C‐positive preadult basal cells around PSG. sp, spinous cells; gr, granular cells; c, cornified cells. Bar in (B) and (J), 50 mm.

absence or presence of 10 nM T3. Not only body epidermal cells but also tail cells were induced to express hbA by T3. A similar response of tail epidermal cells to TH was also reported for Xenopus tadpoles utilizing adult specific

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keratin protein (63 kDa keratin) as a probe (Nishikawa et al., 1992). Apparently, these results indicate that the tail contains a population of cells that is competent to convert to adult epidermal cells in response to TH. Rana tail epidermal cells mostly consist of basal skein cells. Thus, T3‐dependent induction of hbA expression in tail epidermal cells suggests two possibilities. First, very few larval basal cells are included in the tail epidermal preparation, and these cells proliferate and diVerentiate into adult basal cells and then granular cells. Second, basal skein cells will undergo apoptosis under the action of TH in normal development. However, these cells might have the potential to diVerentiate into adult basal cells under appropriate conditions. Subepidermal mesenchymal tissues exert a critical influence in determining an actual diVerentiation pathway from possible diVerentiation potentials. The epidermal cell cultures were freed from subepidermal mesenchymal cells. We assume that basal skein cells are able to diVerentiate into larval basal cells in these conditions. This assumption is based upon studies that show the dependence of the metamorphic fate of larval epidermal cells, either diVerentiation into adult epidermal cells or apoptosis, on the underlying mesenchymal cells (Kawai et al., 1994; Kinoshita et al., 1986a,b). In mammals, the epidermis is constructed by proliferation of epidermal stem cells located on the basement membrane and by diVerentiation of their oVspring. The histological similarity of the adult epidermis between mammals and anurans described in Sections II and III suggests that the anuran basal cells are epidermal germinative (stem) cells. This suggestion is experimentally supported by skin organ culture experiments described in this section.

D. Skin Transformation Center Needle‐like crystals of calcium phosphate are deposited in the upper part of collagen layers of adult bullfrog skin (Taylor et al., 1966). An analysis using an X‐ray microanalyzer confirmed this report (Hayashi et al., 1977). Thus, calcium phosphate seems to be a useful marker of diVerentiation of larval to adult skin. A tadpole at TK‐V was stained with alizarin red S that specifically binds calcium in tissues (Dahl and Dole, 1952). The body skin except the frontal region bound the dye, whereas the tail skin except the anterior region did not bind it (Fig. 8A, Tamakoshi et al., 1998). The red colored region was histologically confirmed to be preadult and the dyeless region to be larval. Thus, whole‐mount in situ staining with alizarin red S is suitable to easily and specifically identify the region where the conversion of larva to preadult was completed. The skin around the boundary region between the body and the tail was removed from a TK‐XXI tadpole and subjected to histological examinations. The top of the collagen layers was stained red by the dye in

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the body side of the skin where the s‐connective tissue had been formed and the epidermis had transformed into adult skin. In sharp contrast the skin on the tail side where the skin remained larval was not stained. Using this method, we sought to determine when and where preadult skin conversion takes place. Tadpoles at various developmental stages were subjected to alizarin red S whole‐mount in situ staining (Tamakoshi et al., 1998). The results are schematically summarized in Fig. 8B. Animals at TK‐II are negative. The red‐colored region first appears at a middle region of both the right and left lateral side at TK‐II to III, indicating that this region is the place where the conversion starts. We postulate a specific site in this middle lateral region where the preadult transformation originates and call this site the STC. The hypothetical STC is the boundary between the stained and unstained region. STC migrates from the original site anteriorly and posteriorly, and dorsally and ventrally, which results in the red staining of the whole body skin

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FIG. 8 Sequential transformation of larval skin into preadult skin. (A) Whole‐mount in situ staining with alizarin red S. A tadpole at TK‐V was stained with alizarin red S. Bar, 1 cm. (B) Schematic representation of the sequential spread of the calcium‐deposited region in the skin. Yellow arrows indicate the direction of the ensuing movement of the skin conversion center.

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A

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FIG. 9 Identification of STC by RAK and SPARC mRNA expression. Back skin sections at TK‐II (larval skin; A, C) and at TK‐IV (preadult skin; B, D) were subjected to H&E staining (A, B) and in situ hybridization of sparc mRNAs (C, D). (A) The larval epidermis faced the thin collagen lamella (cl) under which p‐connective tissues (p‐ct) were present. Basal skein cells (bs; arrowheads) are attached to the basement membrane. Fibroblasts (fb; arrows) are present underneath the acellular collagen lamella. (B) Basal skein cells are replaced with larval basal cells (lb; arrowheads). S‐connective tissues (s‐ct) develop between the epidermis and the thickened collagen lamella. Fibroblasts (arrows) are observed in s‐ct, and in and on the collagen lamella. (C) Basal skein cells (arrowheads) and fibroblasts underneath the collagen lamella (arrows) express sparc intensely in the larval skin. (D) Both larval basal cells (arrowheads) and fibroblasts in and on the collagen lamella (arrows) express sparc. The expression levels are much lower than basal skein cells and fibroblasts in the larval skin. The magnification in (A) and (C) is

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except for the frontal area. The red‐colored region never invades most of the tail region, indicating the presence of a still unknown mechanism that inhibits the migration of STC into the tail. We cloned the SPARC gene as a gene whose expression is upregulated in the larva to preadult skin conversion of R. catesbeiana (Ishida et al., 2003). SPARC is a suppressor of rak during epidermal diVerentiation. mRNA in situ hybridization was performed on sections from larval skin at TK‐II and preadult skin at TK‐IV (Fig. 9). Basal skein cells intensely express SPARC mRNA (Fig. 9C), whereas larval basal cells weakly express it (Fig. 9D). Sections from TK‐IV back skin were subjected to in situ hybridization for rak and sparc (Fig. 9E–G). The examined skin is separated into three regions in terms of rak and sparc expression: (1) the sparc2þ and rak region, (2) sparcþ and rak region, and (3) sparcþ and rakþ region. In the sparc2þ and rak region, sparc is expressed in basal skein cells, and fibroblasts start to migrate into collagen lamella. Thus, the sparc2þ and rak region represents the larval edge. By definition of STC this edge is the larval side edge of STC. In the sparcþ and rak region, basal skein cells greatly decrease sparc mRNA expression, and epidermal basal cells are not committed to express rak yet. These basal skein cells are supposed to diVerentiate into rakþ basal skein cells. Thus, the sparcþ and rak region represents STC. In the sparcþ and rakþ region, the basal skein cells have diVerentiated into rakþ basal skein cells. Thus, the sparcþ and rakþ region is the preadult side edge of STC. H&E staining (Fig. 9E) shows that fibroblasts invade the collagen lamella, but have not developed s‐connective tissue yet. The collagen lamella becomes thinner toward the right side of the view, indicating that the larva to preadult skin transformation progresses to the right. From these observations, we define STC as the sparcþ and rak region. Then, STC is visualized on a histological section as an about 150‐mm‐long region that contains about 20 rak‐ negative and weakly sparc‐positive basal cells (Fig. 9G).

the same as in (B) and (D). Bars, 50 mm. (E–G) Comparison of the expression pattern of rak and sparc. Back skin sections at TK‐IV were subjected to H&E staining (E) and in situ hybridization for rak (F) and sparc (G). (E) Fibroblasts (oblique arrows) often invade the collagen lamella (cl), but s‐ct have not developed between the epidermis and the collagen lamella. The rightmost oblique arrow points to the last fibroblast present in the collagen lamella of the larval region. (F) The rakþ basal skein cells (arrowheads) appear on the left side (preadult region), but not on the right side (larval region). We define the preadult region as the skin in which basal cells are rak þ. (G) Intense signals of sparc mRNA in the epidermis (arrowheads) are observed on the right side, but not on the left side. Fibroblasts are sparc positive. Closed and open thick arrows represent the boundary between the rakþ and rak region and the boundary between the sparc2þ and sparcþ region, respectively. The larval region is defined as the skin in which basal cells are sparc2þ. STC is localized by comparing the expression patterm of rak in (F) and sparc in (G) and sandwiched by the closed and the open thick arrow. STC is progressing toward the right as indicated by the vertical arrow. Bar, 50 mm.

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III. Epithelial–Mesenchymal Interactions and Larval Skin Remodeling A. Tail‐ and Body‐Dependent Metamorphic Fate of Larval Skin STC is the front where larva to preadult skin conversion is actively taking place. STC originates at a specific site of a lateral region of the upper dorsal skin of a larva and migrates to other regions where the larval skin follows ‘‘a diVerentiation program’’ that determines when, where, and how the larval skin diVerentiates to preadult and to adult skin. STC never invades the tail region where larval skin is not transformed to preadult skin, but follows a quite diVerent program, ‘‘an apoptosis program’’ that determines when, where, and how larval skin undergoes histolysis. We are interested in the mechanism under which STC does not invade the tail region. This mechanism is responsible for the region (the tail and body)‐dependent metamorphic fate of larval skin. Previous studies indicate that the mesenchymal compartment plays a critical role(s) in determining the tail‐ and body‐dependent metamorphic fate of larval skin (Kawai et al., 1994; Kinoshita et al., 1986a,b). Both the epidermis and the mesenchyme were isolated from the body (back) and the tail of Rana tadpoles at TK‐IV and X as larval and preadult skin tissues, respectively. There are no histological diVerences between the back and the tail skin at TK‐IV. The basal cells are all basal skein cells and the mesenchyme has not yet developed s‐connective tissue. From these isolated tissues, homo‐ or heterotypically recombined skins were reconstructed and autografted to the back or the tail region to match the site (back or tail) of the epidermis of the recombined skin with that of the recipient. Two types of heterotypic transplants were made: the tail epidermis with the back mesenchyme (T/B) and the reverse (B/T), and two types of homotypic transplant (B/B and T/T). The host animals at TK‐IV and X were allowed to develop for 4 months and 2–3 weeks, respectively, during which the hosts developed to TK‐XIV and XVII. The transplants were subjected to histological and immunohistological investigations. The epidermis of heterotypic grafts in experiments with TK‐IV tadpoles changed its original regionality (dorsum or tail) to a regionality that is identical to the combined mesenchyme: the original tail epidermis in T/B transplants developed into the dorsal epidermis containing preadult basal cells and the original dorsal mesenchyme developed into the dorsal mesenchyme, (i.e., the mesenchyme developed s‐connective tissues and secretory glands, and thickened collagen laminae). Similarly, the original dorsal epidermis in B/T transplants developed as the tail epidermis containing basal skein cells with well developed Figures of Eberth: the attached mesenchyme did not develop s‐connective tissues. Some hosts with

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T/B transplants were allowed to enter the climax stages of metamorphosis. The epidermis became hbAþ, indicating the transplants developed into adult skin. The epidermis of B/T grafts was hbA and its mesenchyme was infiltrated with lymphocytes, indicating that the mesenchyme was under histolysis as originally programmed. In contrast, the epidermis of heterotypically recombined skin made from tadpoles at TK‐X developed as originally programmed. Similarly, no mesenchymal eVects were observed in B/T skin grafts. Thus, it can be said that the body or tail identity of the epidermis is determined by the underlying mesenchyme before the latest TK‐X in bullfrogs. The subepidermal mesenchyme at TK‐X does not possess inductive activity, suggesting that inductive activity is lost when the s‐connective tissue is formed. However, the precise developmental stage at which inductive activity disappears has not yet been determined. It is most likely that mesenchymal inductive ability is lost when basal skein cells are replaced with larval basal cells. Heterotypically recombined skin experiments show that both the body and tail mesenchyme of the larval skin possess inductive ability on the overlying epidermis. However, their ability is quite diVerent in nature: the body mesenchyme induces diVerentiation in the larval epidermis, whereas the tail mesenchyme induces apoptosis in the same tissue. The molecular mechanism for the regionally defined inductive ability of the mesenchyme remains to be determined.

B. Platelet‐Derived Growth Factor (PDGF)‐A Signaling as a Molecular Cue in TH‐Induced Skin Remodeling It is known that epidermal–mesenchymal interactions are also required for the diVerentiation and proliferation of mammalian epidermal cells. PDGF/ PDGFR signaling is claimed to play an important role(s) in this interactive system (Schatteman et al., 1992; Skobe and Fusenig, 1998). The PDGF family consists of four members, PDGF‐A, ‐B, ‐C, and ‐D, each of which assembles into dimers and acts on homo‐ or heterodimers of two receptor tyrosine kinases, PDGFR‐a and PDGFR‐b. PDGFR‐a and ‐b preferentially bind PDGF‐A, ‐B, and ‐C, and PDGF‐B and ‐D, respectively (Betsholtz et al., 2001). The embryonic epidermis and the underlying mesenchymal cells of the mouse skin express PDGF‐A and ‐C and its receptor PDGFR‐a (Aase et al., 2002; Ding et al., 2000; Karlsson et al., 1999; Orr‐Urtreger and Lonai, 1992; Schatteman et al., 1992). PDGFR‐a gene‐deficient mouse embryos often show a severe loss of dermal mesenchyme, which results in the regional detachment of the epidermis (Schatteman et al., 1992; Soriano, 1997). Their epidermal layers are thin and do not develop cornified layers. We tested the possibility that PDGF signaling acts as a molecular cue(s) in the epithelial–mesenchymal interaction in metamorphic skin transformation using X. laevis (Utoh et al., 2003). The skin expresses mRNAs of both

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PDGF‐A and PDGFR‐a at a low level until NF‐56 (premetamorphic stage) and markedly increases the expression at NF‐58 (prometamorphic stage) when the expression is highest and XAK‐C mRNA‐expressing preadult basal cells are first detectable (Watanabe et al., 2002). Then, the level decreases at NF‐60 when tadpoles enter metamorphic climax and the development of s‐connective tissue is complete. mRNAs of XAK‐A and ‐B are first detectable at NF‐60 (Watanabe et al., 2001). The expression of PDGF‐A and PDGFR‐a genes is upregulated by T3, which takes place before XAK‐A and ‐B mRNA‐positive epidermal cells first appear (Watanabe et al., 2001). These correlations between PDGF/PDGFR‐a and XAK‐A, ‐B, and ‐C gene expressions suggest some role(s) of PDGF‐A and PDGFR‐a signaling in T3‐dependent diVerentiation of larval epidermal cells. In situ hybridization experiments on mRNAs of PDGF‐A were done at NF‐57 when larval basal cells are xak‐c . These basal cells do not express PDGFR‐a. The epidermis around NF‐52 contains regions where basal cells have condensed and aggregated. These aggregates develop into PSGs later at early NF‐58 and undergo down‐growth into the dermis to form secretory glands at NF‐59. We consider that larval basal cells near PSGs transform to preadult basal cells because they are xak‐cþ. The preadult basal cells spread to other regions on the basement membrane at late NF‐58 and all the basal cells become xak‐cþ at NF‐59. The xak‐cþ basal cells (preadult basal cells) around PSGs at early NF‐58 express PDGF‐A mRNA, spread on the basement membrane at late NF‐58, and cease to express the mRNAs at NF‐59 when s‐connective tissue is formed. This expression pattern of PDGF‐A mRNAs in larval basal cells indicates that the expression is temporal and closely associated with the diVerentiation of larval basal cells into preadult basal cells. The s‐connective tissue has not formed at NF‐57 and fibroblasts sparsely scattered in the p‐connective tissue weakly express PDGFR‐a mRNAs. Fibroblasts become activated at an early NF‐58, increase their number, migrate into the collagen lamella and to the basement membrane, and begin to form the s‐connective tissue. These fibroblasts are intensely PDGFR‐aþ. Thus, it seems that the expression of the PDGFR‐a gene is correlated with the activation of fibroblasts and with the expression of PDGF‐A mRNAs in preadult basal cells, which strongly suggests some role(s) of PDGF signaling in the epithelial–mesenchymal interaction during the drastic histological change in the metamorphosing skin. In particular, this signaling seems to activate fibroblasts to form s‐connective tissue. This suggestion was tested utilizing an in vitro model of larval skin shown in Fig. 10. Skin pieces were cultured for 9 days in the presence of T3 (control experiments). Skins transformed into the adult type in which cornified cells (Fig. 10A), XAK‐Cþ adult basal cells (Fig. 10B), and XAK‐Bþ suprabasal cells (Fig. 10B) are present. XAK‐Cþ cells are mitotically active (Fig. 10C).

Control

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cl FIG. 10 EVects of inhibitors of PDGF signaling on TH‐induced remodeling of larval skin. Pieces of back skin of tadpoles at stage 54/55 were cultured for 9 days in the presence of 100 nM T3 (þT3). (A–C) Control experiments without inhibitors. (D–F) 10 mM AG1296 was added through the culture. (G–I) 100 mg/ml rECD was present. The skins were subjected to H&E staining (A, D, G) or double immunohistochemical staining for XAK‐B (shown in green) and XAK‐C (red) (B, E, H). The skin tissues in (C), (F), and (I) were exposed to BrdU for the last 24 h and immunostained using anti‐BrdU antibodies. Arrowheads in (C) point to representative BrdU‐ positive cells. Fibroblasts (arrowheads) in (D) and (G) display round and small nuclei indicating possible cell death. The asterisk in (I) indicates nonspecific stains. Dashed lines represent the location of the basement membrane. The abbreviations are the same as in Fig. 7. Bar in (I), 50 mm.

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When added to the cultures, AG1296, a specific inhibitor of PDGFR tyrosine kinase autophosphorylation (Kovalenko et al., 1994, 1997; Levitzki and Gazit, 1995), inhibited the previously described T3‐induced changes (Fig. 10D–F). Similarly, recombinant extracellular domains of PDGFR‐a (rECD) suppressed the TH eVects (Fig. 10G–I). The epidermis fails to develop the multilayers (Fig. 10D and G). In the presence of inhibitors, almost all fibroblasts display round and small nuclei indicating possible cell death (Fig. 10D, G). The invasion of fibroblasts into the collagen lamella is greatly (14‐fold) accelerated by T3. As a result, T3 thickens collagen lamellae about fourfold as compared with T3‐free control cultures. Fibroblasts do not invade the collagen lamella and collagen lamellae do not thicken in the presence of the inhibitors (Fig. 10D, G). The BrdU‐labeling index of basal cells in T3 cultures is 20‐fold higher than that of control cultures. The basal cells with AG1296 (Fig. 10F) and rECD (Fig. 10I) seldom incorporate BrdU, indicating that T3 induces the proliferation of preadult basal epidermis through PDGF signaling. XAK‐Cþ preadult basal cells emerge around PSGs in the absence of TH. Thus, it is most likely that PDGF/PDGFR signaling is not required for the diVerentiation of larval basal cells into XAK‐Cþ preadult basal cells. Actually, both AG1296 (Fig. 10E) and rECD (Fig. 10H) do not significantly aVect XAK‐C expression of basal cells. This signaling is rather required for the initiation of the terminal diVerentiation of adult basal cells, because both inhibited the expression of XAK‐B (Fig. 10E, H). T3 induces these cells to enter the S‐phase of cycles. T3‐activated preadult basal cells seem to diVerentiate into adult basal cells and secrete PDGF, which activates subepidermal fibroblasts. It is clear that PDGF/PDGFR signaling is one of the molecular cues of the epithelial‐mesenchymal interaction required for skin metamorphosis of anurans. At present we postulate that this activation is a key trigger in the formation of s‐connective tissues. It is noteworthy that both PDGF‐A‐ and XAK‐C‐positive basal cells first appear around PSGs at NF‐57 or ‐58. These basal cells increase their number and spread to other regions on the basement membrane. These epidermal events are tightly coupled with the changes in the underlying mesenchyme. The subepidermal fibroblasts underneath the PDGF‐A and XAK‐C‐positive basal cells are highly active in PDGFR‐a mRNA expression as compared with fibroblasts in other regions. We consider that these subepidermal fibroblasts are in an ‘‘activated’’ state and are participating in constructing the s‐connective tissues. PDGF/PDGFR signaling plays a role in activating the fibroblasts. PDGF/PDGFR signaling plays key roles in epithelial–mesenchymal interaction during mammalian skin development. The overexpression of PDGF‐A in epithelial grafts induces the formation of thicker and more cellular connective tissues (Eming et al., 1995, 1998). When PDGF‐overexpressing human

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keratinocytes were transplanted onto the back of nude mice, dermal fibroblasts became activated to proliferate and, in turn, the host epidermis also became proliferative and abnormally multilayered, probably due to some paracrine factor(s) secreted by the activated fibroblasts (Skobe and Fusenig, 1998). Conversely, PDGF‐A / mice (Karlsson et al., 1999) and Patch mutation mice whose PDGFR‐a gene is deleted (Schatteman et al., 1992) develop thinner dermal tissues and skin devoid of the dermis, respectively.

C. The Skin of Vertebrates: Evolutional Significance of Anuran Skin Metamorphosis In the previous sections we described the transformation of aquatic larval skin to a terrestrial adult counterpart. In this section the histological features of both types of anuran skin are compared with those of other vertebrate species as an approach to understanding the evolutional significance of anuran skin metamorphosis. The vertebrate epidermis is derived from the ectoderm and is homologous in basic histological structure among amniotes (reptiles, birds, and mammals), termed the stratified squamous epithelium (Matoltsy and Huszar, 1972). The epidermis of amphibia shares a basic structure with amniotes, suggesting that the animals evolved the epidermis that adapted the terrestrial habitation at the emergence of ancestral amphibia and has conserved its basic structure through humans. The epidermis of these animal species is composed of basal, spinous, granular, and cornified layers, each of which is located sequentially upward from the most inner cell layer (the basal layer). The basal and the spinous layer together represent the germinative layer, constitute the proliferative compartment, and are collectively called the stratum Malpighii. The progenies yielded upon division of the cells therein move upward losing replicative capacity up to the cornified layer in which the cells become terminally diVerentiated anuclear cornified cells. The basal layer in mammals represents a compartment where epidermal stem cells are located (Fuchs and Serge, 2000; Watt and Hogan, 2000). The mammalian epidermal stem cells have been well characterized and represent a specific population of basal cells attached to a unique site of the basement membrane (Jones and Watt, 1993; Jones et al., 1995). The definition of a stem cell indicates that upon cell division a stem cell produces two daughter cells, one being a copy of the mother cell (self‐renewal) and the other being transit amplifying cells (TA cells) that produce more diVerentiated cells upon cell divisions (Watt, 2002). Thus, the stem cell and its descendant diVerentiated cell are said to be in a hierarchic relation. Upon cell division TA cells yield first the spinous cell, which then yields the granular cell. The granular cell yields the cornified cell. As the hierarchic position goes up, the proliferative potential decreases, spinous cells being highest, whereas the extent of diVerentiation

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increases, cornified cells being in the terminally diVerentiated state and finally sloughing oV as anucleated cells. This kind of hierarchic system in epidermal cells is considered to have first emerged in amphibia in which the stratum corneum is thought to have evolved about 350 million years ago (Matoltsy and Bereiter‐Hahn, 1986). We term this type of epidermis ‘‘the single‐lineage epidermis’’ in this review. The epidermis is attached to the basement membrane that binds to the mesoderm‐derived dermis. The dermis plays roles in regulating the proliferation and diVerentiation of the epidermal cells and, thus, epithelial–dermal interactions are critical in the development and physiology of the skin. Figure 11 schematically compares the development of skin between mammals and amphibians, using Mus musculus and X. laevis as a representative example of each of the classes, respectively. A mouse embryo at E10 of gestation is covered with the ectoderm underlain with the mesoderm. At E12 the ectoderm develops into the epidermis composed of two layers, the periderm at the top and the basal layer at the bottom. Periderm and basal cells autonomically recycle, (i.e., when periderm cells are lost, nearby periderm cells divide and replace them) (Bickenbach and Holbrook, 1986, 1987; Holbrook, 1991). The epidermis at E15 becomes multilayer containing intermediate layers between the periderm and the basal layer. The mesenchymal fibroblasts form the dermis. Intermediate cells are considered to be descendants of basal cells and are in a diVerent lineage from the periderm (Matoltsy, 1986). Thus, the epidermis at this developmental stage is a ‘‘two‐lineage epidermis.’’ At birth the epidermis forms the basic structure of the adult‐ type epidermis with hierarchical layers from basal to cornified layers. The periderm cells undergo apoptosis and are sloughed oV (Boneko and Merker, 1988), indicating that the epidermis transforms from a two‐ to a single‐ lineage epidermis. The epidermis is combined with the mesoderm‐derived dermis. The X. laevis skin progressively changes its histological structures during metamorphosis (Fig. 11). The epidermis at NF‐30 (tail bud stage) is two‐ layered, the outer cell and inner cell layers, the cell in the outer layer being ciliated. The epidermis has developed to a ‘‘larval epidermis’’ at NF‐45 that is composed of apical and basal skein cell layers. The collagen lamella, a histological entity unique to amphibian dermis, has developed, which is combined with the p‐connective tissue. At the middle larva stage (around NF‐55), small basal skein cells have emerged at the basal layer. Larvae do not significantly change this structure until the prometamorphic stage (NF‐58 to ‐59) when basal skein cells diVerentiate into larval basal cells, and the s‐connective tissue is formed between the collagen lamella and the basement membrane. The skin drastically transforms its histology into an adult form during climax stages of metamorphosis (NF‐60 to ‐64), by diVerentiating larval basal cells into adult counterparts, and simultaneously deleting

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Cilia Outer cell Inner cell p-connective tissue Apical cell Basal skein cell Collagen layer

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Spinous cell Adult

Adult basal cell

FIG. 11 Schematic representation of the development of skin in mammals (Mus musculus) and anurans (Xenopus laevis). Stages of skin development are represented by days after coitus (E) for mice and conventional terms of developmental stage for anurans. The histology of mouse skin at E10, E12–E15, and birth corresponds to that of anuran skin at early embryonic, larval, and froglet stages, respectively. The epidermis develops to a ‘‘larval epidermis’’ at NF‐45, which is composed of apical and basal skein cell layers. The collagen lamella (collagen layer) develops, which is combined with the p‐connective tissue. At a middle larva stage (NF‐55), small larval basal cells have emerged at the basal layer. Larval basal cells are well developed at the prometamorphic stage (NF‐58 to ‐59) and the s‐connective tissue is formed between the collagen lamella and the basement membrane. The skin drastically transforms its histology into an adult one during the climax stages of metamorphosis (NF‐60 to ‐64), larval basal cells diVerentiating into adult ones.

apical and suprabasal skein cells. The skin of froglets shows the adult histology composed of multilayered epidermis with the dermis consisting of the s‐connective tissue, the collagen lamella, and the p‐connective tissue.

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The epidermis shows the histological feature characteristic of mammals. Thus, it can be said that the anuran transforms a two‐lineage to a single‐lineage epidermis during metamorphosis. The comparison of developmental changes between M. musculus and X. laevis suggests that apical cells are homologous to periderm cells. This assumption is supported by the fact that apical cells express an anuran homologue of cytokeratin 8 (CK8) (Suzuki et al., 2001), a marker of periderm cells (Moll et al., 1982). Histological features suggest that the integument of a late embryo at the tail bud stage (NF‐30) to an early larva around NF‐45, a larva at NF‐45 to NF‐58, and a froglet of X. laevis corresponds to that of M. musculus at 12, 15, and birth, respectively. It is intriguing to assume that the developmental stage of mammalian skin when periderm cells are deleted corresponds to the metamorphic climax of amphibian skin. Fish are placed in the phylogenetic tree as the most primitive vertebrate. Fish is a polyphyletic term including nontetrapod vertebrates (lampreys, sharks and rays, actinopterygians, coelacanths, and lungfishes) and hangfish. In this review the word fish is used to refer to actinopterygian fish and in particular teleosts, because developmental changes have been most studied at histological and gene expression levels for the zebrafish (Danio rerio) (Le Guellec et al., 2004). The fish epidermis is quite diVerent from the other tetrapod epidermis. Generally, the fish epidermis is composed of three layers: the outermost, the intermediate, and the basal layer (Whitear, 1986). The superficial cells are not cornified. The intermediate layer per se is multilayered and contains various secretory cells such as goblet, club, and sacciform cells, and these cells are seemingly undiVerentiated. DiVerent from the tetrapod epidermis, it seems that there is no hierarchic relationship among the cells in the three layers. Each cell type is mitogenic, and divides autonomically when surrounding cells are accidentally damaged and lost (Le Guellec et al., 2004). In other words, the basal cells in fish are not the source for cells in the upper layers. Thus, it can be said that the epidermis of teleosts is a ‘‘multilineage epidermis.’’ In addition, interestingly from this review’s point of view, skein cells are present in the basal layer of lamprey epidermis (Lane and Whitear, 1980) as in amphibian. There is a similarity in the dermal structure between the fish and the amphibian. The unique plywood‐like collagen lamella is present in fish dermis and directly contacts the subepidermal basement membrane. Fish basal cells synthesize and secrete type 1 collagen, which is deposited subepidermally as the collagen lamella. The collagen lamella is originally acellular, but later is populated by fibroblasts that participate in the formation of the collagen lamella and are responsible for its development and maintenance after the epidermal cells cease to express the collagen gene. No connective tissues are present between the basement membrane and the collagen lamella in early development after hatch. Although the s‐connective tissue‐like structure is

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formed by fibroblasts, it is very scanty. These histological features of the fish skin are remarkably similar to those of anuran larval skin. On the other hand, the histological features of the adult anuran skin are basically identical to those of tetraploid vertebrates. Therefore, it is tempting to speculate that the metamorphosis of the anuran skin is a process that might have taken place when ancestral amphibians were evolved from fish approximately 350 million years ago.

IV. Genes Involved in Anuran Tissue Remodeling A. Unique Utilization of TH Response Element in Metamorphosis‐Associated Genes Anuran metamorphosis represents a biological process in which larval tissues are replaced with adult ones under the control of TH. The replacement proceeds in a complex but exquisite manner, requiring precise TH‐ dependent spatiotemporal regulation of epithelial–mesenchymal interactions. It is evident that many metamorphosis‐associated genes participate in this tissue remodeling. Genes play prime roles whose expressions are under the direct control of TH. TH exerts its actions by binding with the nuclear TR, a transcriptional regulator. TR binds to the TRE present in a TH‐direct responsive gene, together corepressors and coactivators of transcription. Thus, the elucidation of factors involved in TH‐TR‐TRE signaling and their roles are a central issue to the understanding of metamorphosis at the molecular level. Matrix metalloproteinases (MMPs) play major roles in removing old tissues by degrading extracellular matrices. More than 25 human MMPs and the homologue from other species have been identified (Egeblad and Werb, 2002). The larval tissue is ‘‘the old tissue’’ to be removed in metamorphic remodeling (Yoshizato, 1989). Stromelysin‐3 (MMP‐11) is involved in the remodeling of larval intestine (Ishizuya‐Oka et al., 2000; Patterton et al., 1995). Genes of collagenases are upregulated in metamorphosing X. laevis tadpoles (Berry et al., 1998; Stolow et al., 1996; Wang and Brown, 1993). Gelatinase A (MMP‐2) and B (MMP‐9) are induced in T3‐treated tadpole tails (Jung et al., 2002). MMP‐1 degrades type I collagen, which is the most abundant collagen in animal tissues. Tissue inhibitor of metalloproteinase (TIMP), a specific inhibitor of collagenase, and a synthetic MMP inhibitor, Ilomastat, inhibits TH‐induced tail regression (Oofusa and Yoshizato, 1991) and retards tail resorption (Jung et al., 2002), respectively. The expression of the MMP‐1 gene and its protein is especially high in degrading tail tissues during metamorphosis (Oofusa and Yoshizato, 1991).

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Comparisons of sequences and the exon structures of cDNA between amphibian and mammalian MMP1 suggested that R. catesbeiana MMP‐1 (rMMP1) is an ancestral form of mammalian MMP1 (Oofusa and Yoshizato, 1994). Western and Northern blot analyses showed that the enzyme is upregulated by TH at both protein and mRNA levels (Oofusa and Yoshizato, 1991, 1994, 1996). The rMMP1 gene (rmmp‐1) contained a TRE sequence (50 ‐AGGTAA‐ GAACAGGATA‐30 ) from 891 to 876. We determined if the rmmp‐1 TRE sequence functions in living cells (Sawada et al., 2001). A plasmid, pEGFP/rmmp‐1 ( 1078/þ98), was constructed that contains a 50 ‐upstream region ( 1078 to þ98) of rmmp‐1 as a promoter and enhanced green fluorescent protein (EGFP) cDNA as a reporter. The back and the tail lateral skin of Rana tadpoles at TK‐X each was transfected with the plasmid. The animals were reared in the presence of T3. The expression of EGFP increased T3 dose dependently as high as 7‐fold over that in the absence of the hormone, indicating that the TRE sequence in rmmp‐1 is a biologically active TRE in vivo. We questioned whether rmmp‐1 contains sequences that regulate TRE activity. The rmmp‐1 gene contains an ‘‘AP‐1 and Sp‐1’’ region at 99 to 15, which serves as the basic promoter for the initiation of transcription in the human gelatinase gene (Huhtala et al., 1991). Double‐stranded oligonucleotides termed AS ( 99/þ98) were synthesized that contained an AP‐1 and Sp‐1 region and were used as a basic promoter. Similarly, two oligonucleotides were synthesized, TRE ( 891/ 876) and TREf ( 891/ 840), which consisted of TRE ( 891/ 876) and its 30 ‐flanking 36 bp ( 875/ 840). Each TRE ( 891/ 876) and TREf ( 891/ 840) was ligated to AS ( 99/þ98) at its 50 ‐terminus, the product of which was inserted into pEGFP. Thus, we prepared three vectors, pEGFP/ TRE ( 891/ 876)/AS ( 99/þ98), pEGFP/TREf ( 891/ 840)/AS ( 99/þ98), and pEGFP/TREf ( 891/ 840). Tadpoles were bombarded with each of these vectors to determine their TH responsiveness. Among them only TREf/AS significantly responded to T3. Thus, both the flanking 36 sequence and the ‘‘AP‐1 and Sp‐1 region’’ are together required for TRE to respond to T3. The 36‐bp‐long direct 30 ‐flanking sequence might be necessary for the function of TRE, acting as its activator. The human MMP1 gene (accession numbers AF023338 and D26110) does not contain either the direct repeat or the palindrome type of TRE in the nucleotide sequence database within its 1 kb upstream region, but one such sequence of direct repeat 4 (DR4, TGACCCTCAGAGACCT) is present if the search is extended to 10 kb ( 7057 to 7072). Similarly, there is one DR4 sequence (TTACCTCAGGTAAACT) in the chicken (Gallus gallus) MMP1 gene at 9476/ 9461 and four DR4 sequences in the MMP1‐ like gene of fish, Tetraodon nigroviridis. However, there have been no studies to test whether such sequences of DR4 function as TRE. The databases of the genomic gene of MMP1 of reptiles are not available at present. Under these current situations of genomic databases and functional tests, it is too

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early to argue the biological significance of the presence of TRE in anuran MMP1 in relation to metamorphosis. However, it is tempting to speculate that the TRE in anuran MMP1 was uniquely evolved to regulate the remodeling of larval to adult tissue during metamorphosis as previously discussed (Oofusa and Yoshizato, 1991, 1996). A diVerent ‘‘modification’’ in the TRE‐related transcriptional system was reported for the MMP9 gene, which seems to be uniquely evolved in amphibians (Fujimoto et al., 2006). Two types of gene for MMP‐9, which cleaves native type IV collagen, were cloned from Xenopus tropicalis and X. laevis: the conventional type (MMP‐9 gene) and a unique one (MMP‐9TH gene). These genes are located tandemly about 9 kb apart from each other in the genome. The MMP‐9TH gene was expressed in the regressing tail and gills, and the remodeling intestine and central nervous system, whereas MMP‐9 mRNA was detected in embryos. TH upregulates the MMP‐9TH gene through three TREs that are located in the distal promoter and the first intron. It has been suggested that the MMP‐9 gene is duplicated and diVerentiated into two genes, one of which, MMP‐9TH, is specialized in function to work in TH‐dependent degenerating and remodeling processes during metamorphosis. Such duplication of MMP‐9 has not been found in other vertebrate genomes reported to date. Germline transgenetic tadpoles of X. laevis (Kroll and Amaya, 1996) have been utilized to test whether genes actually play a role in regulating metamorphosis. For more than three decades PRL had been considered to be an important endocrine acting as an antagonist of metamorphosis. Transgenetic tadpoles bearing the PRL gene showed no delay in normal tadpole life, indicating PRL does not play a role in metamorphic processes (Huang and Brown, 2000b). Interestingly, they became ‘‘tailed frogs,’’ suggesting that the growth of fibroblasts in the tail was stimulated. This outcome supported our previous observation that PLR stimulates collagen synthesis of tail fibroblasts (Yoshizato and Yasumasu, 1970). The autoregulation of the TR gene by T3 was first suggested by our previous study in which the aYnity of TH to the nuclear TR was determined in tail cell nuclei prepared from tadpoles at various stages of metamorphosis (Yoshizato and Frieden, 1975). In fact, the Xenopus TRb (xTRb) gene contains TRE in its transcriptional regulatory region (Ranjan et al., 1994; Wong et al., 1998). A functional assay of TRE was made utilizing Xenopus oocytes and A6 cells, a cell line derived from the kidney of Xenopus. A fusion gene consisting of a TRE‐containing 50 ‐flanking region of the xTRbA1 gene and a reporter gene was injected into the oocytes or the cells. The expression of the reporter gene was upregulated in response to T3 (Ulisse et al., 1996). Using the gel shift assay Shi and his colleagues demonstrated the binding of heterodimers, xTRb/Xenopus retinoid X receptor a (xRXRa) or xTRb/xRXRg, to a TRE‐containing sequence of the xTRbA1 gene (Ranjan et al., 1994; Wong

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and Shi, 1995). These studies show that the binding of a complex of T3 and xTRb/xRXR heterodimers to the promoter region of the xTRb gene is a key event in inducing anuran metamorphosis. To understand the role of TH‐TR‐TRE signaling in the development of amphibians in vivo we investigated EGFP expression patterns in transgenic Xenopus tadpoles carrying xTRbA1 gene promoter‐driven EGFP cDNA (Oofusa et al., 2001). Visceral tissues including the intestine and the pronephra become prominently fluorescent at around NF‐42, with the expression level increasing until NF‐45 and then decreasing gradually thereafter. Nervous tissues are strongly fluorescent at NF‐42 and ‐45. The tail muscle shows a high level of EGFP expression from NF‐42 to ‐57. The muscle of hind limbs becomes intensely fluorescent at NF‐54, its intensity greatly increasing at the climax stage of metamorphosis. After metamorphosis, the fluorescence becomes gradually weaker in all the tissues described previously. When these tadpoles reach the climax stage (from NF‐58 to ‐60), the fluorescence regains a high intensity. It is most likely that these high levels of expression during metamorphic climax are induced by T3, because it is well established that the plasma level of T3 becomes high (Leloup and Buscaglia, 1977). When treated with T3, transgenic tadpoles at NF‐51 evidently increase fluorescence at 5 days in all tissues, especially in the jaw, the nervous tissues, the body muscles, the pronephra, the forelimbs, the hind limbs, and the muscle of the tail. The previously described overall expression profile of the xTRb promoter‐ driven reporter gene during larval development supports the results of previous reports that studied the expression of xTRb mRNA by in situ hybridization (Kawahara et al., 1991) and reverse transcriptase‐mediated hybridization (Yaoita and Brown, 1990). A markedly high expression of the reporter gene in T3‐treated tadpoles was seen in nervous tissues, jaw, gills, thyroid gland, small intestine, liver, and tail muscle. These organs, except the thyroid gland and the jaw, have been reported to be TH responsive by Ishizuya‐Oka et al. (1996) for small intestine, Kawahara et al. (1989) for liver, Hu et al. (1999) for tail muscle, Atkinson (1981) for gills, and Buckbinder and Brown (1992) for brain. Thus, we concluded that the transgene containing the TRE sequences responds well to T3 in TH‐responsive tissues of spontaneous and TH‐induced metamorphosing tadpoles in a biologically meaningful manner. In addition, two new aspects of TH‐TR‐TRE signaling were revealed. It has been generally thought that TH in amphibians functions only as a metamorphosis‐inducing hormone, since the discovery that tadpoles fed on thyroid glands precociously metamorphose (Gudernatsch, 1912). This notion has been supported by the fact that TH in sera is detectable only from just before and during the climax stage of metamorphosis. TH has not been thought to play roles in embryogenesis and in adult tissue physiology. The results obtained from experiments with xTRbA1 gene‐transgenic X. laevis do

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not agree with this general belief. Unexpectedly, but interestingly, we observed the first significant EGFP fluorescence in embryos at NF‐14 (the neurula stage) (Fig. 12). Reporter protein expression was intense in the upper half of the neural fold. Western blotting for xTRb gave an immunopositive band for embryos at NF‐14. These results together strongly suggested that TH‐TR‐TRE signaling plays a role(s) in anuran embryogenesis, especially in neural tube formation. This suggestion is important, because first, it is known that TH is necessary for the normal development of the brain in mammals (Forrest et al., 2002; Koibuchi and Chin, 2000; Yen, 2003) and second, embryos at this stage have not yet developed functional thyroid glands. It is known that TR acts as a suppressor of the transcription of TRE‐containing genes when unligated and as a stimulator when ligated (Mahajan and Samuels, 2005). Thus, the question of whether TH is present in anuran embryos is critical.

A

D

B

C

E

FIG. 12 Expression of EGFP in embryonic neural folds in transgenic Xenopus tadpoles carrying xTRbA1 gene promoter‐driven EGFP cDNA. Eggs with transgenes were developed to NF‐14 (A, B, C) and ‐30 (D, E), and photographed from a side of the animal pole under a bright (A) and fluorescent field (B, D). Photos of (A) and (B) are from the same embryo and from the same direction. Sections (C) and (D) were stained with anti‐EGFP antisera. The dorsal side is up in (C) and (E). The anterior side is to the left in (E). The arrows in (C) indicate the immunoreactive regions. All the tissues in (E) are immunopositive. Bars, 1 mm.

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There has been a study that showed its presence. Radioimmunoassay detected both T3 and T4 in toad (Bufo marinus) embryos (Weber et al., 1994). These hormones are likely of maternal origin. It was also reported that the TRa gene is expressed in developing oocytes (Kawahara et al., 1991). Its mRNA is present throughout embryonic development (Eliceiri and Brown, 1994). Thus, it is plausible that TH‐TR‐TRE signaling plays a key role(s) in embryonic neural fold formation. There have been few studies on the physiological role of TH in amphibia after metamorphosis. The TH responsibility of the TRE‐containing gene in adult tissues was examined by bathing the 4‐ to 8‐week‐old transgenic frogs in T3‐containing water. EGFP fluorescence became brighter. The fluorescence started to increase 1 day after hormone treatment and reached a plateau at 2 days when the intensity rose 1.6‐fold as compared to controls. Our study showed that TRE‐containing promoters are also responsible for exogenous TH in adult tissues, especially in the brain, intestine, bones of the upper forelimbs and the foot of the hind legs, and kidney as well as neighboring tissues. These results strongly suggested that TH might play some role in these tissues of adult frogs. It is well known that TH generally stimulates the basic metabolic activity of cells in adult mammalian tissues (Yoshizato et al., 1980). In particular, oxygen consumption of brain, liver, kidney, and muscle significantly increases in TH‐treated adult rats (Frieden and Lipner, 1971). Mundy et al. (1976) showed that TH directly stimulates the resorption of rat long bones in organ culture. Therefore, it is likely that TH regulates these processes in adult frog tissues as in mammals. Galton (1985) reported the presence of T3‐binding sites in nuclei of liver cells and erythrocytes of adult frogs, although their number is significantly lower than that of tadpoles, which also supports the notion that adult anuran cells respond to T3 to some extent. Based upon the results obtained from the TRb gene‐ transgenesis studies, we propose that TH‐TR‐TRE signaling is essential not only for the progression of metamorphosis, but also for embryogenesis and adult physiology. We could obtain a more general view to understand the biological significance of TH in amphibians by studying its role not only in metamorphosis, but also in embryogenesis and adult tissue physiology.

B. Regulation of Gene Expression in Larval Tissue Remodeling TH triggers metamorphosis of anurans, the process in which all larval organs are remodeled to adult ones (Gilbert and Frieden, 1981; Shi, 1999; Yoshizato, 1989, 1996). Isolated pieces of tail or the whole tail in culture undergo histolysis in the presence of TH (Tata et al., 1991; Weber, 1967). Similarly, isolated larval intestine tissues in culture alone undergo remodeling to an

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adult tissue when TH is provided (Ishizuya‐Oka and Shimozawa, 1991). These studies suggest that each of the larval organs is remodeled autonomically. Such autonomy is also shown for larval skin transformation in this review. On the other hand, organs and tissues of a tadpole each interdependently metamorphoses: there are the ordered sequences of remodeling of organs. For example, metamorphosis of the limb takes place earlier than that of the tail. Skin metamorphosis is another example of such an ordered sequence. As detailed in Section V, the appearance and migration of STC are well organized in that STC emerges at a specific site and at a specific stage of larval development, and moves in a developmental stage‐ and region‐ dependent manner. STC never travels into the tail domain. This orderly proceeding of metamorphosis of each organ as a whole gives the impression that there is a surveillance system that determines the ordered sequence of metamorphosis of an organ. Tadpoles undergo drastic changes in their body structure and function in a very elegant and exquisite manner at every step of metamorphosis and in a harmonious and concerted way as a whole. TH initiates anuran metamorphosis and regulates the ensuing whole process. Therefore, the responsiveness of cells to TH is essential for tadpoles to initiate metamorphosis and for it to progress. Thus, the previously mentioned organized procession of remodeling of each organ can be explained by the diVerent aYnities of constituent cells of an organ toward TH. For example, limb cells might show a higher aYnity to TH than tail cells. To our knowledge, there have been no studies that comparatively and quantitatively examined the aYnity of each larval tissue cell in a systematic and comprehensive manner. The responsiveness of a cell to TH is basically determined by either its binding capacity or binding aYnity toward TH. It is thought that the sensitivity of a cell of larval tissue is maximal at the climax stage of metamorphosis when the TH concentration in blood is at its maximum. Changes in the maximal binding capacity and the binding aYnity of tail cell nuclei were determined at various stages of development and metamorphosis of tadpoles by Scatchard analysis (Yoshizato and Frieden, 1975). The result supports the idea that the maximum number of binding sites rather than the aYnity of a larval cell is correlated with the cell’s responsiveness to TH. If this conclusion can be extended to larval cells of other tissues, it can be generally said that the expression level of the TR gene of a cell is a good measure to assess its sensitivity to TH. Therefore, it will be valuable to comprehensively compare experimental data on the expression level of TR genes among various types of larval cells, and during the time course of development and metamorphosis to understand the ordered sequence of metamorphic changes of larval tissues. Cellular responsiveness or nonresponsiveness to TH is determined by whether a cell possesses TRs or not. TRs act as thyroid hormone acceptors

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by making heterodimers with 9‐cis‐retinoic acid receptors (RXRs). Thus, the regulation of expression of genes of TR and RXR in a cell is essential for the cell to respond to TH. Practically, TR gene expression is a determinant of cellular responsiveness to TH, because RXR is constitutively expressed during the development and metamorphosis of tadpoles (Wong and Shi, 1995). Genomic DNA of four types of TRs (TRaA, TRaB, TRbA, and TRbB) was cloned from X. laevis and characterized in relation to their roles in metamorphosis (Brooks et al., 1989; Yaoita et al., 1990). It has been thought that TRb plays a prime role(s) in inducing metamorphic changes, because the expression level of this gene correlates well with the rise in the level of an active form of TH, T3 in blood during metamorphosis (Yaoita and Brown, 1990). Utilizing transgenesis technology, it was shown that the intracellular TR level is a determinant of cell sensitivity to TH (Schreiber and Brown, 2003). TRa binds to TH and coactivators through its carboxyl 401 amino acid residues. Deletion of this region yields a dominant negative form of TRa (TRDN). cDNA (Ker:TRDN) was constructed in which TRDN was incorporated under the control of a promoter sequence of keratin gene that is exclusively expressed in apical epidermal cells. The investigators made transgenic tadpoles bearing this construct. Tissues and organs of the transgenic tadpole generally underwent normal metamorphosis except tissues in the skin. The larval epidermal basal cell normally transformed into the adult basal cell and the subepidermal mesenchyme converted to the adult type. However, apical cells did not undergo apoptosis, but survived in the adult skin. This result clearly demonstrates two things. One is that TR is critical for TH‐dependent metamorphosis. The other is that each of the skin cells individually responds to TH and autonomically metamorphoses into the counterpart of adult skin cells. TRE present in a transcription regulatory region of a gene is another determinant of the cell’s responsiveness to TH. Generally, the expression of hormone‐responsive genes is regulated by the ligand (hormone)‐activated receptors (ligand–receptor complex) that bind to cis‐acting elements in the regulatory region of target genes (Evans, 1988; Yamamoto, 1985). TRE is such an element for TH‐targeted genes. When the T3/TR/RXR/TRE complex is formed in a cell, the cell potentially becomes responsive to TH. Thus, it is helpful for us to comprehensively list all the genes that contain TRE. If a gene possesses TRE in its transcription regulatory region, we assume that the gene is potentially of prime importance for the initiation and progression of metamorphosis. Actually, TRE was found in a flanking region of the start site of the X. laevis thyroid hormone receptor b (TRb) gene (Ranjan et al., 1994). The transcriptional expression of stromelysin‐3 is under the direct control of TH, because TH induces its expression within a few hours in the absence of protein synthesis (Damjanovski et al., 2000). However, a TRE has yet to be identified in its genomic DNA (Li et al., 1998). Regulatory regions

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of xBTEB were shown to contain TRE (Furlow and Brown, 1999). TRE has been shown in several mammalian genes, genes of malic enzyme (Petty et al., 1990), myosin heavy chain (Flink and Morkin, 1990), and growth hormone (Sap et al., 1990). The complete list of TRE‐containing genes in anurans and a comparison with that in mammals will greatly aid us in understanding the organized procession of metamorphosis. When available, such a list for all classes of vertebrates will be valuable in understanding the biological and evolutional significance of metamorphosis at the molecular level. Furthermore, the list will contribute to determining the suggested ‘‘hierarchical gene network’’ that substantiates the ordered and concerted sequences of metamorphosis of larval tissues. There is an additional factor that determines the sensitivity of larval tissues for TH. The concentration of TH in blood is high at climax stages of metamorphosis, indicating that every larval tissue is evenly exposed to a high level of TH then. However, most (approximately 90%) of the TH in blood is T4, the prohormone of T3. T4 should be deiodinated to be the active TH, T3. One of the critical factors that determines the responsiveness of a cell to TH is an ‘‘eVective intracellular concentration’’ of TH. The deiodination reaction is catalyzed by deiodinase (Leonard and Visser, 1986). Currently, three types of deiodinase are known: DI, D2, and D3. The former two types convert T4 to T3 and the last type deletes iodo at the 5 position of the inner ring of T4 to T3, resulting in the inactivation of T3. The presence of D2 and D3 deiodinase was reported in anuran tissues (Becker et al., 1997). The D3 deiodinase gene is TH responsive and upregulated by the hormone (Wang and Brown, 1993). Thus, the intracellular eVective T3 concentration is determined by the intracellular concentration of D2 and D3 enzymes if the ambient concentration of TH is constant. Several studies have supported this prediction. The retina of tadpole in premetamorphic stages grows by proliferating symmetrically at the ciliary marginal zone (CMZ). However, the CMZ increases in size ventrally but not dorsally from the prometamorphic to climax stages (Beach and Jacobson, 1979a). Thus, the majority of the adult frog retina is derived from ventral CMZ cells. This shift from symmetrical to asymmetrical growth is TH dependent (Beach and Jacobson, 1979b; Hoskins and Grobstein, 1985). The asymmetrical TH‐dependent growth of CMZ cells was explainable by the expression of type III deiodinase in dorsal but not ventral CMZ cells (Marsh‐Armstrong et al., 1999). Type III deiodinase‐transgenic tadpoles were yielded, in which the transgene was under the control of a panactive promoter, CMV, or a neural‐specific promoter prepared from the neural b‐tubulin gene. These tadpoles did not show the TH‐induced proliferation of the ventral CMZ cells (Huang et al., 1999; Marsh‐Armstrong et al., 1999). A fusion gene of green fluorescent protein (GFP) and D3 was incorporated into a vector with a CMV‐IE94 promoter/ enhancer. Germline transgenic tadpoles bearing this construct were produced,

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which ubiquitously expressed the D3 enzyme at a high level, the enzyme activity being more than 20‐fold that of normal larvae. The transgenic tadpoles normally developed limbs before the climax stage, but most of them terminated metamorphic progress at an early climax stage of metamorphosis (NF60/61), and died with gills and tail. This study shows that limbs are sensitive to TH and are able to develop under a minute level of T3, whereas the tail’s sensitivity is low and requires a high level of T3 to normally metamorphose. It seems that the metamorphic transformation of cells basically proceeds autonomically and interdependently. The present review describes the latter in detail, focusing on the interaction between epidermal and mesenchymal cells taking place during skin metamorphosis. We can predict the presence of a gene network (‘‘metamorphosis gene network’’) in which each of the constituent genes is turned oV or on interdependently and in a harmonized manner in response to TH directly or indirectly, or in response to a factor induced by cell–cell communications. At first glance, each of the on/oV switches takes place autonomically in each of the cells. However, when we see a tadpole as a whole, the ability of the gene to turn on/oV apparently takes place in a finely ordered manner mainly through the diVerence in an eVective local concentration of T3, an amount of available TR in a cell. The elucidation of the entire structure of this metamorphic gene network is necessary to comprehensively understand the mechanism of metamorphosis, but this is likely to require some years.

V. Concluding Remarks The metamorphic transformation of anuran larval skin to adult counterparts has been a major target of our research activities aimed at revealing the mechanism of metamorphosis at histological, cellular, protein, and gene levels. The epidermal and dermal cells were characterized based on their role during this process by examining their morphological and histological features, the expression profiles of genes and proteins, and the interdependence between epidermal and dermal cells. As a result we were able to identify a unique site termed the skin transformation center (STC), in which larval skin is actively undergoing a transformation into adult skin. PDGF/PDGFR signaling was found to play a role(s) as one of the cues for the epithelial–mesenchymal interactions in the body‐ and tail‐dependent metamorphic transformation of larval skin. As a result of these studies we have noticed that the skin of an aquatic anuran larva and a terrestrial anuran adult is histologically analogous to that of an aquatic adult of fish and a terrestrial adult of tetrapod, which suggests the evolutionary significance of anuran metamorphosis. TH‐TR‐TRE signaling plays a major role in

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regulating metamorphic skin transformation. Based upon studies on the transcriptional regulation of TH‐responsive genes, we propose a new view of the biological role of TH in anurans: TH‐TR‐TRE signaling plays a significant role not only in the development and the metamorphosis of larvae as ‘‘the metamorphic hormone,’’ but also in embryogenesis as a ‘‘morphogen’’ of neural fold formation and in adult tissue physiology as a ‘‘metabolism‐ modulating hormone.’’ This viewpoint leads us to compare the results obtained from studies on the anuran as a metamorphic animal with those on other vertebrates as nonmetamorphic animals, which will eventually enable us to understand the uniqueness and generality of anuran metamorphosis. A cell responds to TH through TH‐TR‐TRE‐signaling and, thus, the extent of the cell’s responsiveness is determined by intracellularly available concentrations of both TH and TR. Individual larval cells autonomically undergo biochemical reactions to TH when concentrations of the ligand and its receptor are appropriate. Therefore, the elucidation of the mechanism by which their eVective concentrations are determined will be necessary to understand the metamorphosis of a tadpole, in which cellular events proceed in a well orchestrated manner following finely ordered sequences.

Acknowledgments This review is dedicated to my mentor, the late Professor Koscak Maruyama (1930–2003), who guided me when I started my research as a graduate student, encouraged me during my research activities, and advised me through my career as a biologist. The author thanks Drs. Y. Ishida, K. Suzuki, K. Oofusa, and R. Utoh for their kind cooperation during the preparation of this manuscript. The studies described in this article were supported by a Grant‐in‐Aid for Scientific Research A (07404057, 2000–2002) and B2 (15370028, 2003–2005).

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Further Reading Amano, T., Kawabata, H., and Yoshizato, K. (1995). Characterization of metamorphic changes in anuran larval epidermis using lectins as probe. Dev. Growth DiVer. 37, 211–220. Ataliotis, P., Symes, K., Chou, M. M., Ho, L., and Mercola, M. (1995). PDGF signaling is required for gastrulation of Xenopus laevis. Development 121, 3099–3110. Collier, I. E., Smith, J., Kronberger, A., Bauer, E. A., Wilhelm, S. M., Eisen, A. Z., and Goldberg, G. I. (1988). The structure of the human skin fibroblast collagenase gene. J. Biol. Chem. 263, 10711–10713. Fini, M. E., Plucinska, I. M., Mayer, A. S., Gross, R. H., and BrinckerhoV, C. E. (1987). A gene for rabbit synovial cell collagenase: Member of a family of metalloproteinases that degrade the connective tissue matrix. Biochemistry 26, 6156–6165. Flamant, F., and Samarut, J. (1998). Involvement of thyroid hormone and its alpha receptor in avian neurulation. Dev. Biol. 197, 1–11. Huang, H., and Brown, D. D. (2000a). Overexpression of Xenopus laevis growth hormone stimulates growth of tadpoles and frogs. Proc. Natl. Acad. Sci. USA 97, 190–194. Kinoshita, T., and Sasaki, F. (1994). Body‐specific proliferation of adult precursor cells in Xenopus larval epidermis. Histochemistry 101, 397–404. McCawley, L. J., and Matrisian, L. M. (2001). Matrix metalloproteinases: They’re not just for matrix anymore! Curr. Opin. Cell Biol. 13, 534–540. Takada, M., Yai, H., and Takayama‐Arita, K. (1995). Corticoid‐induced diVerentiation of amiloride‐blockable active Naþ transport across larval bullfrog skin in vitro. Am. J. Physiol. 268, 218–226. Takada, M., Shiibashi, M., and Kasai, M. (1999). Possible role of aldosterone and T3 in development of amiloride‐blockable SCC across frog skin in vivo. Am. J. Physiol. 277, 1305–1312.

INDEX

A Activin primordial germ cell proliferation regulation in testis development, 129 somatic cell proliferation regulation in testis development, 138 AlkB, substrate specificity, 84 AMH, See Anti-Mu¨llerian hormone Anti-Mu¨llerian hormone comparative sexual diVerentiation, 115–117 culture studies of testicular development, 154–155 peritubular myoid cell migration regulation in testicular development, 123–124 Sertoli cell phenotype and diVerentiation control, 147–149 signaling, 124 Antley-Bixler syndrome, cytochrome P450 reductase missense mutations, 55–56 APUD cell, stomach in swine, 6

B BDNF, See Brain-derived neurotrophic factor Benzene, metabolism, 84 Benzo(a)pyrene, metabolism, 84–85 Bilirubin formation, 67–69 UDP-glucuronosyltransferase metabolism Crigler-Najjar syndrome and hyperbilirubinemia, 71 gene therapy for hyperbilirubinemia, 71–73

261

glucuronidation and excretion into bile, 69–70 Gunn rat and hyperbilirubinemia, 70–71 hyperbilirubinemia defects, 67, 70–71 overview, 67 Biliverdin reductase, bilirubin formation, 68 BMPs, See Bone morphogenetic proteins Bone morphogenetic proteins male germ cell phenotype/diVerentiation control, 141–142 testicular vascular morphogenesis role of BMP-2, 127–128 Brain-derived neurotrophic factor, peritubular myoid cell migration regulation in testicular development, 125

C Calmodulin, nitric oxide synthase reductase domain regulation, 53–54 Carboxylesterase, substrate specificity, 82 Cholecystokinin, secretion in swine, 9 Cilia human disease defects, 179–181 length control therapeutic targeting, 203–204 structure and composition, 179 Cnk2, flagellar length control, 200 Collagen, metamorphosis in anuran skin, 220, 222 Crigler-Najjar syndrome, hyperbilirubinemia and UDP-glucuronosyltransferase defects, 71

262

INDEX

Cytochrome P450 aromatic compound metabolism, 84–85 CYP26B1 in male sexual development, 140–141, 154 gene organization, 88 NADPH-cytochrome P450 reductase/ cytochrome P450 system catalytic cycle of reductase, 47 electron transfer system evolutionary aspects, 44–47 FAD/FMN pair regulation, 52–55 mechanism, 47–51 reductase domain structure, 39–43 functional interactions, 75–78 history of study, 37–38 molecular oxygen activation by P450, 51–52 overview, 36–37 reductase missense mutations in Antley-Bixler syndrome, 55–56 subcellular localization, 73–74 topology, 75 substrate specificity, 81–82 UDP-glucuronosyltransferase interactions, 79–81

D Desert hedgehog, Leydig cell diVerentiation control, 150–151 Diaphorase, See NAD(P)H:quinone oxidoreductase Dopamine, quinone toxicity, 87 Drug-metabolizing enzymes, See specific enzymes

E Endocrine cells, stomach in swine, 7–9 Endoplasmic reticulum, size control studies, 177 Epithelial–mesenchymal interaction, See Metamorphosis, anuran skin Epoxide hydrolase, substrate specificity, 82–83 ER, See Endoplasmic reticulum Esophagogastric ulcer epidemiology, 2–3 etiopathogenesis, 10–15

history of study, 2 mucin changes, 13–15 peptic ulcer similarity, 2 stomach morphofunctional features in swine, 3–10 Estrogens, metabolism, 85

F FGF, See Fibroblast growth factor Fibroblast growth factor Leydig cell diVerentiation control, 152 primordial germ cell migration regulation in testicular development, 119–120 proliferation regulation in testicular development, 130–131 Sertoli cell phenotype and diVerentiation control by FGF-9, 144–145 somatic cell proliferation regulation in testis development, 133–135 Flagella assembly, 181–182 defects and human disease, 179–181 length control advantages as model system for organelle size, 177–178, 204–206 Chlamydomonas mutants identification, 189 intraflagellar transport, 190–191 long-flagella mutants, 189–190 overview, 178–179 protein localization and function, 191–192 control models balance point model, 198–203 cumulative strain model, 195–197 feedback model, 197–198 molecular ruler model, 192–194 quantal production of limiting precursor model, 194–195 distribution, 182–184 equalization following perturbation, 186–188 nanotechnology prospects, 207 regeneration, 184–186 structure and composition, 179 Flavin proteins, See Cytochrome P450; Nitric oxide synthase

263

INDEX Follistatin, testicular vascular morphogenesis role, 127–128 Frog metamorphosis, See Metamorphosis, anuran skin

G

I IFT, See Intraflagellar transport Integrin b1, metamorphosis in anuran skin, 220, 222 Intraflagellar transport Chlamydomonas mutants, 190191 flagella assembly, 181–182 particle aggregate studies, 201–203

G cell, stomach in swine, 7–8 Gastric acid, secretion in swine, 9–10 Gastrin, secretion in swine, 9–10 GDF-9, See Growth diVerentiation factor-9 GDNF, See Glial-derived neurotrophic factor Gene therapy, UDP-glucuronosyltransferase targeting for hyperbilirubinemia, 71–73 Glial-derived neurotrophic factor (GDNF) male germ cell phenotype/diVerentiation control, 144 primordial germ cell proliferation regulation in testis development, 132 Sertoli cell phenotype and diVerentiation control, 150 somatic cell proliferation regulation in testis development, 138–139 Glutathione S-transferase, drug metabolism, 36 Growth diVerentiation factor-9, male germ cell phenotype/diVerentiation control, 142–143 GST, See Glutathione S-transferase Gunn rat, hyperbilirubinemia and UDPglucuronosyltransferase defects, 70–71

Leptin, male germ cell phenotype/ diVerentiation control, 143 Leukemia inhibitory factor, primordial germ cell proliferation regulation in testis development, 130 Leydig cell, diVerentiation and phenotype control Desert hedgehog, 150–151 fibroblast growth factor, 152 platelet-derived growth factor, 151–152 LIF, See Leukemia inhibitory factor

H

M

Helicobacter pylori, esophagogastric ulcer induction, 11, 27 Heme oxygenase (HO), bilirubin formation, 67–68 Hepatocyte growth factor peritubular myoid cell migration regulation in testicular development, 122–123 Sertoli cell phenotype and diVerentiation control, 146–147 somatic cell proliferation regulation in testis development, 135 HGF, See Hepatocyte growth factor Histamine, esophagogastric ulcer induction, 13 HO, See Heme oxygenase Hyperbilirubinemia, See Bilirubin

MAPK, See Mitogen-activated protein kinase Matrix metalloproteinase, metamorphosis in anuran skin, 243–245 Metamorphosis, anuran skin basal cell precursor studies Rana catesbeiana tadpole, 224–225, 227 Xenopus laevis tadpole, 228–230 epidermal cell molecular markers, 220–222 epithelial–mesenchymal interactions platelet-derived growth factor signaling, 235–236, 238–239 tail- and body-dependent metamorphic fate, 234–235 evolutionary significance, 216, 239–243 overview, 217–220

K Keratins esophagogastric ulcer changes, 20 metamorphosis in anuran skin, 217, 221, 225, 227–228

L

264

INDEX

Metamorphosis, anuran skin (continued) region-dependent progression of remodeling, 214–215 skin transformation center, 230–231, 233 thyroid hormone role gene expression regulation in larval tissue remodeling, 248–252 overview, 215–217, 225, 227, 229–230 platelet-derived growth factor mediation, 235–236, 238–239, 252 response element utilization by metamorphosis-associated genes, 243–248, 253 Mitogen-activated protein kinase, flagellar length control, 192, 198 MMP, See Matrix metalloproteinase Morphogenesis, See Testicular morphogenesis Mucins esophagogastric ulcer changes, 13–15 stomach in swine, 5–6 Mucosa keratinization in esophagogastric ulcer, 17–20 stomach in swine, 4

N NAD(P)H:quinone oxidoreductase mechanism, 86 substrate specificity, 83 Nerve growth factor discovery, 113–114 peritubular myoid cell migration regulation in testicular development, 125 somatic cell proliferation regulation in testis development, 139 Neurotrophins peritubular myoid cell diVerentiation control, 153 migration regulation in testicular development, 125 primordial germ cell proliferation regulation in testis development, 132 Sertoli cell phenotype and diVerentiation control, 150 signaling, 125 somatic cell proliferation regulation in testis development, 138s NGF, See Nerve growth factor

Nitric oxide synthase isoforms and functions, 41 reductase domain electron transfer, 40 evolutionary aspects, 44–47 FAD/FMN pair regulation, 52–55 NADPH-cytochrome P450 reductase homology, 39, 42 structure, 40–43 turnover numbers, 54 NOS, See Nitric oxide synthase NQO1, See NAD(P)H:quinone oxidoreductase

O Organelle size control flagella, See Flagella study examples, 176–177

P PDGF, See Platelet-derived growth factor Pepsin, secretion in swine, 9 Peritubular myoid cell, migration regulation by growth factors anti-Mu¨llerian hormone, 123–124 hepatocyte growth factor, 122–123 neurotrophins, 125 platelet-derived growth factor, 120–122 transforming growth factor-b, 123 PGC, See Primordial germ cell Phase I enzymes, See Cytochrome P450 Phase II enzymes, See also UDP-glucuronosyltransferase substrate specificity, 81–83 types, 36 Platelet-derived growth factor isoforms, 120 Leydig cell diVerentiation control, 151–152 peritubular myoid cell diVerentiation control, 152 migration regulation in testicular development, 120–122 primordial germ cell proliferation regulation in testis development, 131–132 Sertoli cell phenotype and diVerentiation control, 145–146

265

INDEX somatic cell proliferation regulation in testis development, 135 thyroid hormone-induced skin remodeling role in anurans, 235–239, 252 Primordial germ cell male germ cell phenotype/diVerentiation control bone morphogenetic proteins, 141–142 glial-derived neurotrophic factor, 144 growth diVerentiation factor-9, 142–143 leptin, 143 overview, 139–141 transforming growth factor-b, 142 vascular endothelial growth factor, 143–144 migration in testicular development, 118–120 Protocadherin, gene organization, 63

R Reserpine, esophagogastric ulcer induction, 13, 15–16, 19

S SCF, See Stem cell factor SDF1, See Stromal cell-derived factor 1 Secretin, secretion in swine, 9 Sertoli cell phenotype/diVerentiation control anti-Mu¨llerian hormone, 147–149 fibroblast growth factor-9, 144–145 hepatocyte growth factor, 146–147 neurotrophic factors, 150 platelet-derived growth factor, 145–146 transforming growth factor-b, 149–150 proliferation regulation in testis development activin, 138 fibroblast growth factor, 133–135 hepatocyte growth factor, 135 neurotrophic factors, 138–139 overview, 132–133 platelet-derived growth factor, 135 transforming growth factor-a, 135–136 transforming growth factor-b, 136, 138 Sexual diVerentiation, comparative biology, 114–118

Skin, See Metamorphosis, anuran skin Skin transformation center, anuran skin metamorphosis, 230–231, 233 SOX9, comparative sexual diVerentiation, 115, 118 SRY, comparative sexual diVerentiation, 115, 118 STC, See Skin transformation center Stem cell facto, primordial germ cell proliferation regulation in testis development, 129–130 Stomach clinical spectrum, 22–23 diVerential diagnosis, 23 forensic evaluation, 24–27 morphofunctional features in swine, 3–10 pathomorphology macroscopic findings, 15–17 microscopic findings, 17–22 treatment and prophylaxis, 24 Stromal cell-derived factor 1, primordial germ cell migration regulation in testicular development, 119 Sulfotransferases drug metabolism, 36 substrate specificity, 83 Swine, See Esophagogastric ulcer

T Testicular morphogenesis cell migration germ cells, 118–120 interstitial cells and growth factor regulation anti-Mu¨llerian hormone, 123–124 hepatocyte growth factor, 122–123 neurotrophic factors, 125 platelet-derived growth factor, 120–122 transforming growth factor-b, 123 comparative biology, 114–118 culture systems for growth factor studies, 153–158 germ cell phenotype/diVerentiation control bone morphogenetic proteins, 141–142 glial-derived neurotrophic factor, 144 growth diVerentiation factor-9, 142–143

266 Testicular morphogenesis (continued) leptin, 143 overview, 139–141 transforming growth factor-b, 142 vascular endothelial growth factor, 143–144 Leydig cell diVerentiation control Desert hedgehog, 150–151 fibroblast growth factor, 152 platelet-derived growth factor, 151–152 peritubular myoid cell diVerentiation control neurotrophin, 153 platelet-derived growth factor, 152 primordial germ cell proliferation regulation activin, 129 fibroblast growth factor, 130–131 leukemia inhibitory factor, 130 neurotrophic factors, 132 platelet-derived growth factor, 131–132 stem cell factor, 129–130 transforming growth factor-b, 128–129 prospects for growth factor studies, 158–161 Sertoli cell diVerentiation control and testicular cord formation anti-Mu¨llerian hormone, 147–149 fibroblast growth factor-9, 144–145 hepatocyte growth factor, 146–147 neurotrophic factors, 150 platelet-derived growth factor, 145–146 transforming growth factor-b, 149–150 somatic cell proliferation regulation activin, 138 fibroblast growth factor, 133–135 hepatocyte growth factor, 135 neurotrophic factors, 138–139 overview, 132–133 platelet-derived growth factor, 135 transforming growth factor-a, 135–136 transforming growth factor-b, 136, 138 vascular development overview, 125–127 regulation bone morphogenetic protein-2, 127–128 follistatin, 127–128 vascular endothelial growth factor, 127

INDEX TGF-a, See Transforming growth factor-a TGF-b, See Transforming growth factor-b TH, See Thyroid hormone Thyroid hormone, anuran skin metamorphosis role gene expression regulation in larval tissue remodeling, 248–252 overview, 215–217, 225, 227, 229–230 platelet-derived growth factor signaling mediation, 235–236, 238–239, 252 response element utilization by metamorphosis-associated genes, 243–248, 253 Transforming growth factor-a, somatic cell proliferation regulation in testis development, 135–136 Transforming growth factor-b male germ cell phenotype/diVerentiation control, 142 peritubular myoid cell migration regulation in testicular development, 123 primordial germ cell migration regulation in testicular development, 120 proliferation regulation in testis development, 128–129 Sertoli cell phenotype/diVerentiation control, 149–150 somatic cell proliferation regulation in testis development, 136, 138

U UDP-glucuronosyltransferase aromatic compound metabolism, 84–85 bilirubin metabolism overview, 67 hyperbilirubinemia defects, 67, 70–71 glucuronidation and excretion into bile, 69–70 membrane topology and transport, 69–70, 78–79 Gunn rat and hyperbilirubinemia, 70–71 Crigler-Najjar syndrome and hyperbilirubinemia, 71

267

INDEX gene therapy for hyperbilirubinemia, 71–73 cytochrome P450 interactions, 79–81 drug metabolism, 36 evolutionary aspects, 64–67 functional overview, 56–57 gene organization, 61–63, 88 history of study, 57–58 structure and function, 59–61 subcellular localization, 73–74 substrate specificity, 81–82 UGT, See UDP-glucuronosyltransferase

V Vascular endothelial growth factor male germ cell phenotype/diVerentiation control, 143–144 testicular vascular morphogenesis role, 127 VEGF, See Vascular endothelial growth factor Vitamin E, esophagogastric ulcer prophylaxis, 24 Vitamin U, esophagogastric ulcer prophylaxis, 24